RECIST 1.1: Principles, Pearls, and Pitfalls, Dr. Lacey McIntosh (10-1-25)
HIDEInteractive Transcript
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Hello and welcome to Noon Conference, hosted by Modality
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Noon Conference connects the global radiology community
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through free live educational webinars that are accessible
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for all and is an opportunity
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to learn alongside top radiologists
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from the around the world.
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Today we are honored to welcome Dr.
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Lacey Macintosh for a lecture entitled,
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resist 1.1 Principles, pearls and Pitfalls.
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Dr. McIntosh is an associate professor
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of radiology at UMass Medical Schools
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and specializes in cancer and molecular imaging.
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She currently serves as the associate program director
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of Diagnostic Radiology Residency and Chief of Oncology
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and Molecular Imaging at UMass Memorial Medical Center.
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She loves teaching and working with residents.
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At the end of the lecture, please join her in a q
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and a session where she will address questions you may
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have on today's topic.
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Please remember to use that q
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and a feature to submit your questions so we can get to
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as many as we can before our time is up.
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With that, we are ready to begin today's lecture.
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Dr. McIntosh, please take it from here.
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Great. Thank you, Ashley,
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and thanks for inviting me to speak on this topic.
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Um, so today, as she mentioned,
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we're gonna talk about recess 1.1 principles,
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pearls and pitfalls.
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Um, I do some consulting for clinical trial reads
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and curriculum content creation.
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Um, so the objectives of this lecture are to
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increase overall familiarity
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with Resus 1.1 response assessment criteria, um,
1:26
to really understand the concepts behind this, uh,
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and to integrate the principles into clinical care when, uh,
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we're reading studies on cancer patients.
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So the purpose of Resus, like why do we have these, uh,
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tumor response assessment criteria?
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And the goal is that we really want to determine if
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and how well an anti-cancer agent works.
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Um, and the goal with these is to have these designed
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to be the most accurate way
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to capture the treatment response.
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Um, so Resus 1.1 is probably the most popular
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and the one that people are most familiar with,
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but it's, um, and it's often
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but not always the most appropriate, uh,
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response assessment criteria for a particular cancer
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or a particular drug.
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Um, and like many of these assessment criteria,
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this has evolved over time.
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Once people start using it, they find, um, you know, uh,
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gaps or holes and ways to improve it.
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So the current, the most, um, current iteration
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that we use is this recess 1.1 over here on the right.
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Now, as I mentioned, resist is not the only assessment
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criteria, but it's one of many.
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Um, I listed here a table
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that shows some other response criteria.
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For example, these ones are used in, uh,
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renal cell carcinoma,
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but other ones that you may have heard of might be choi, um,
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immune related response criteria, mass criteria, um,
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lugano is one that's used for lymphoma.
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So, um, if we have time at the end, I'll, I'll sort
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of touch on some of these as well,
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but reist is just one of, of many,
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but it's probably the most commonly used for solid tumors.
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Um, so we must acknowledge like, yes, the goal
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of looking at these assessment criteria is to find a way to
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quantify something that's very qualitative, right?
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Looking at imaging. Um,
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and so we do that by measuring things and describing things,
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but, uh, we must acknowledge
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that not all disease is really amenable to being measured.
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Um, and so there are other, you know, systems that we use
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to try and assess, um, tumor volumes
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and tumor burden, um, even when they can't be measured.
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So I just wanted to mention this one.
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This is the peritoneal carcinomatosis index.
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And so, um, this is another way that people sort of use to
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quantify how much peritoneal disease there is.
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As, as you guys know, it can be very difficult to measure,
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but, um, this is achieved by splitting the abdomen,
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abdomen up into these, um, different sections,
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and then providing a score based on
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how much disease you see in each area.
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Alright, so Resis 1.1.
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Um, most radiologists I think are aware of this
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and have heard about it, but, um, you know,
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we aren't really using this at the workstation on patients
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every day unless you're participating in, um, you know,
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assessing patients who are on clinical trials.
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Um, but, you know, many
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of us are reading cancer studies at the workstation
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and not really using recess in a formal way.
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Um, these are used in clinical trials.
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They, you know, follow a very strict sort of, um,
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guideline of how they're done.
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And, um, you know,
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imaging is done on a very particular schedule.
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So when, when this is used in the setting
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of a clinical trial, it's very formal.
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Um, you know,
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even though you're not using at the workstation,
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I think it's a really important thing for radiologists
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to be aware of, because
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what we're doing at the workstation is really based off of,
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um, of resist.
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Uh, we're doing it in a little bit different way.
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We're combining it with clinical factors.
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We have a lot more information about, you know,
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what's going on with the patient.
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We have notes from the me, the electronic medical record
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that we can sort of integrate.
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We have tumor markers, all those sorts of things.
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But, you know,
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performing actual formal resus reads at the workstation
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can be challenging, right?
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Um, patients travel around for care and outside,
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or baseline imaging may not be available,
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especially if you work at a, a referral center
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where patients are coming from other places.
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Um, as I mentioned,
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the imaging is done on a pretty strict schedule time-wise,
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um, and it's, you know, designed to assess, uh,
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treatment at certain intervals.
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And, um, as we all know for various reasons,
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patient preference
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or, uh, you know, patient, um,
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on a patients that we need to scan, um, at our centers
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and, you know, contrast, availability, all of these things,
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um, you know, it's not always possible
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to get patients' imaged on a certain timeline in the,
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in the practical clinical setting.
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Um, you know, and finally, time, it takes time
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to do these formal, um, these formal assessments.
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And we all know that time is not in surplus, um,
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for us radiologists these days.
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But, um,
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and as I mentioned, not, uh,
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resus isn't used in all cancer types.
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Um, and we will talk about some of these at the end
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of the presentation, but lymphoma, just on gle, um,
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mesothelioma are just a few examples where
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Resus doesn't really, um, isn't the best
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and most accurate way to capture tumor burden and response.
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So this is an overview table,
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and we're gonna sort of dive into all
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of these things in the next part of the lecture.
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But, um, the top part sort of talks about how we define
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and select disease that we're going to track over time.
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Um, so we look at targets
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and we, these can be non nodal, like a tumor,
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a liver met a lung lesion, um,
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and those are gonna be measured in your long axis.
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Uh, in order to qualify as a target, it has
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to be one centimeter or greater.
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Um, these can also be lymph nodes, which, um, these need
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to be, uh, these need to measure 1.5 centimeters
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or greater in the shortest axis.
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Um, and these are measured routinely on the axial,
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that's the convention is measuring in the axial plane.
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So, um, we just give one
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to measure one dimensional measurements here.
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Um, thing for disease that are, are not targets, um,
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these are things that are either non-measurable
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or, um, in excess of your target lesions.
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Um, the nodes can be a little bit smaller,
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but the short axis must still be greater
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than one centimeter.
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Um, and then we, we formally follow up to five lesions total
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and two lesions max per organ.
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Lymph nodes globally count as one organ,
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so you can only measure
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and follow two, uh, target lymph nodes,
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even if they're from different parts of the body.
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Um, and then we calculate a sum of the target diameters.
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Um, and so we, we create an assessment based on sort
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of what's going on with our targets and our non-arts,
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and then we track these over time.
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So the bottom part of the graph
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or the table shows, um, then we assign, you know,
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these different response categories to, uh, each time point.
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And so, um, you know, the ideal situation is
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that we see a complete response
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where we have a disappearance of all disease,
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and lymph nodes don't really
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disappear when they're involved.
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So they, we just require those to normalize,
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and that's defined as having a short axis
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of one centimeter or less.
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Um, when we see a 30%
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or more decrease in the sum of diameters compared
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to baseline, um, that's considered a partial response.
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And then I'm gonna skip down to progressive disease.
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This is a 20%
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or greater increase in the sum of diameters compared
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to the Nader or where disease looked the best.
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And I, I've got a slide on this later.
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Um, and this must be an absolute increase
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of five millimeters or greater.
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You don't wanna be calling progression on a lymph node
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that's increased in, you know, two or three millimeters.
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And then stable disease is, um, really sort of a catchall
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that, um, encompasses anything that falls
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between a PR and a pd.
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Um, so the, the language is really sort of particular, um,
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you know, uh, stable disease can really allow
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for quite a bit of improvement
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and quite, you know, a, a bit of, uh, worsening as well
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and still be considered stable disease.
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So that's something to sort of be aware of.
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Alright, a general workflow
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for a patient in a clinical trial
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that's being assessed on by Resus.
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1.1 is, you know, determination of eligibility.
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Um, this is usually done by CT MRI can also be used.
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Some of the, um, you know, they,
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the language in Resus 1.1 talks about the role
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of chest x-ray, but honestly, in modern day cancer imaging,
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there really isn't much of a role for chest x-ray.
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Um, PET can also be used as a substitute or an adjunct.
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Um, but CT is really preferred where you can do, um,
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measurements on the axial plane.
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That can be done, um,
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sequentially the same way on subsequent, um, studies.
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So targets are then chosen,
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and we'll talk about this in the next couple slides,
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and we calculate the sum of the diameters, um,
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and then we identify non-arts
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and sort of describe those, uh, create a report
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and then, um,
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patients are followed up at subsequent time points.
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And this can be different from study, from trial to trial.
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So principles, all disease must be accounted
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for on your baseline scan.
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Um, so you're gonna go through
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and select your appropriate targets
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and like we said, up to five targets, two max per organ.
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And then everything else is gonna be a non-target.
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Um, and you can follow these individually or in groups.
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Um, I tend to be a grouper.
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An example of this would be if you had, you know,
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10 liver metastases, you would maybe select the two largest
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and easiest to reliably measure,
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and you'll use those as targets.
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And then you must have a group of non-target,
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or you must have non-arts
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to follow the remaining liver lesions.
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And so I would probably create a group that was, you know,
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non-target number, whatever it is,
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and say remaining liver lesions,
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and then you follow those as a group.
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Um, it's important to classify all
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of your disease at baseline, um,
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because as you follow it, you, you need to be able
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to formally track everything.
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So in the example that I gave,
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if you have multiple liver lesions, only two
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of which are targets, if one of the ones
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that has not been designated as a target starts to grow
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or progress, you can't really call that new disease.
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That's not accurate.
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Um, it's really,
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it would be progression in off target disease.
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So, um, you just need to make sure
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that everything is classified either as a target
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or non-target, um,
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that you've determined represents disease at baseline.
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Um, so when selecting your targets, you usually wanna go
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for the largest lesions
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and ones that like really represent your disease.
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Um, however, uh, if these are not really amenable
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to measurement or they, um, are not, you know, going
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to be reliably measured between from study to study,
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you know, bowel lesions can be really difficult.
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You can imagine on axial plane,
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a bowel lesion may look very different, um,
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from study to study.
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So that's sort of the judgment call of the reader.
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Um, but usually you wanna do the largest, easiest
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and most reliable to measure at subsequent time points.
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Um, and then as I mentioned, you're going
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to either report the long axis if it's a non nodal lesion
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or the short axis if it's, uh, a mal, a lymph node
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that you believe to be malignant.
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Um, and then nodes that are,
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we see this all the time clinically, right, like nodes
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that are less than 10 millimeters.
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We definitely see these nodes that are involved, especially
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with, you know, things like rectal cancer
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or, um, you know, lesions that we see on PET
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that are FDG avid and clearly involved,
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but don't quite meet this.
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And so that's another differentiation of, you know,
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doing this, uh, using Resus versus like your clinical reads.
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Um, the point of Resus is to track and measure
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and to, you know, quantify disease volumes, uh,
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or disease, um, diameters
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and sort of look at, uh, levels of improvements.
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So you may have to ignore lesions that you, um, you know,
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you suspect could be involved,
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but if they're not really, if they don't fall into this
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trackable category, you have to just sort of let them go.
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Um, that's not really the goal of, of recess is
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to catch everything,
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but it's to catch everything that's, um, you know,
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obviously disease and trackable.
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So some considerations.
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If you have a lesion that has a hypervascular rim, you want
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to include that in your measurement.
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Um, bony disease is generally not appropriate as a target.
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Um, and the reason for that is
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because we're tracking size over time, right?
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And if you have a, a bone lesion, um, you know,
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and you're measuring it, bone lesions when they heal,
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often become more sclerotic
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and they don't necessarily disappear.
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So you can imagine that even if your bone lesion like
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totally heals, you're not gonna have,
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you're not gonna have a significant change
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in the size of it.
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And so Resus isn't really gonna capture that response.
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So if your lesion has a significant soft tissue component,
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your bone lesion does, you can select that as a target.
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Um, but anything
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that's really bone based should be a non-target lesion
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and not, not be considered target.
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So after you've selected your targets, you're gonna
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classify everything else, um, as non-arts.
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And so these may be, you know, just whatever is in excess
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of your targets, but also things that aren't suited
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for exact measurements but can be followed.
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So things like effusion, ascites, um, lepto ingal disease,
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lymphangitis involvement of the skin or the lung.
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Here's an example here
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of lymphatic carcinomatosis of the lung.
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We have some ascites.
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We've got sclerotic bone or some sort of mixed lytic
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and sclerotic bone disease here.
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And so you're gonna categorize that baseline
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that this is just like present.
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You wouldn't really categorize it as absent
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'cause you wouldn't be listing it as as a lesion.
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So it's just at baseline,
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it's given the designation of present.
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Um, other things
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that might be appropriate non-arts are lesions
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that have been ablated or radiated.
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Um, and yeah, that's just something to sort of think about.
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Generally, you're not supposed to ch
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to choose these as targets.
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Um, some clinical trials have exceptions and allow for that.
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Um, you know,
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especially if it's like the only site of disease as well.
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So at baseline, you're gonna calculate your sum
15:45
of diameters using the long axis for non nodal lesions
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and the short axis for nodal lesions.
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Here's an example here.
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Um, we've got multiple liver lesions
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and we've selected two that we're measuring in the longest,
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um, diameter on the axial plane.
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Um, we've got a lymph node here, um,
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which is being measured in the short axis,
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and then a peritoneal mass, uh,
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or two peritoneal masses here in the
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pericolic gutter and pelvis.
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And so you'd, um, get the measurements from all
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of these and add them up.
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So some places use like a, a chart like this
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where you can sort of put everything in, um, you need
16:21
to provide series and image numbers for reference as well.
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Um, and then you're gonna calculate your sum of diameters,
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you're gonna talk about your non-target lesions,
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and then any other findings that may be, you know, sort
16:34
of present or contributory or just incidental.
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Um, your baseline report, you know,
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is gonna include normal things like the modality
16:41
and the parameters, use slice thickness, all of that.
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Um, you're gonna talk about your target lesions with ser
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with series and image numbers, um,
16:50
and then non-target lesions as we mentioned,
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and incidental findings.
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Uh, and then you're gonna come up with a conclusion.
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So moving up for, into follow up, um,
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you wanna make sure sort of,
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you wanna do your quality assessment to start like,
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you know, is this follow-up study technically
17:09
comparable to the prior.
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Um, you know, as I mentioned, we really like
17:12
to do CT versus ct.
17:15
We really prefer contrast CT and contrast ct,
17:18
but as you guys know, patients can't always get contrast
17:21
and you know, sometimes they get other
17:22
imaging for other reasons.
17:24
So that's again,
17:25
a judgment call on the reader if the subsequent imaging is
17:29
an appropriate and, um, you know, comparable study to use,
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um, if it's a,
17:35
an appropriate substitute for adequate assessment.
17:39
And then you're gonna go through your targets
17:41
and you're gonna calculate the sums
17:43
of diameters on your new study.
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Um, you wanna continue to measure lymph nodes even if they,
17:48
when they drop below one centimeter
17:50
and they're considered normal, um, you still want
17:53
to document, you know, those single
17:56
millimeter uh, measurements.
17:57
And the reason is that you don't want to, uh, if
18:00
that lymph nodes begins to en enlarge again,
18:02
and, you know, say it goes up
18:04
to like 12 millimeters short axis, if you've documented that
18:07
as a zero previously, that's going
18:09
to overstate the progression versus if it went from nine
18:12
millimeters to 12 millimeters.
18:14
Um, and you can have a complete response even if your sum
18:18
of diameters isn't zero, if you have nodal lesions, um,
18:22
you're gonna assess your nont targets
18:24
and you're gonna say, you know, are they present?
18:27
Are they absent? Are they present with progression?
18:29
Have they worsened? Um,
18:31
and then of course you're gonna look
18:32
for any new sites of disease.
18:34
So here's some examples here where, um, we had some lesions
18:39
that, you know, are very, very small to begin with,
18:41
and then on follow up they're getting bigger.
18:43
So you're gonna measure those.
18:45
Um, and then new liver lesions here on the bottom study.
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Uh, and then here on the right we can see we've got,
18:55
you wanna measure these in the same as
18:57
as much in like a similar manner, a reproducible manner.
19:01
Um, that may not always be possible if
19:04
where the long axis is changed, uh, has changed,
19:08
but you really want to try to do that.
19:10
So this is a lung lesion that's decreased in size,
19:13
another one in the right lung.
19:15
And then, um, you can see there's like a little bit
19:17
of a change in orientation of the SubCal lymph node,
19:20
but you're still sort of in the spirit
19:21
of measuring it in the same short axis there
19:26
sometimes lesions, um, split or merge.
19:30
Um, and so we have, you know, sort
19:32
of accommodations to figure that out.
19:34
If your lesion has split into two lesions, it, you know,
19:36
turns out it was a conglomerate to begin with
19:38
or for whatever reason, it's splits.
19:40
You basically treat these two lesions as one lesion
19:44
and you, um, you add their, their diameters together
19:48
to be able to compare it to the prior.
19:50
Um, and then same thing when lesions sort
19:53
of become confluent.
19:54
Um, you treat those, that group of lesions as
19:57
as a single one, and you try to, you know,
19:59
make the measurements as comparable as possible.
20:02
Um, sometimes like non nodal lesions will become too small
20:05
to measure if they're like, you know, 1, 2, 3 millimeters
20:09
and those are given an arbitrary
20:11
measurement of five millimeters.
20:13
Um, some other things that can happen with certain drugs
20:16
as you can see cavitation.
20:17
Um, and that can be a little bit, you know, difficult
20:20
to document and figure out like,
20:22
how do we measure this, right?
20:24
And we'll talk about this later,
20:25
but that, that is something that's a little bit
20:27
of a pitfall for reis, right?
20:29
Because the overall size
20:30
of this lesion hasn't really changed.
20:32
But, um, you can certainly see
20:33
that there's less tumor there.
20:36
Um, here's an example of a lesion
20:38
that's maybe become too small to measure.
20:40
It's just sort of like a scar.
20:44
And then when you're following up your non-arts, um,
20:47
you're often not measuring.
20:48
I mean you can if they're measurable lesions
20:50
and you can sort of look at that and track that,
20:52
but you're not really calculating anything based on
20:55
non-target measurements.
20:57
Um, you're really just giving more
20:59
of a qualitative assessment.
21:00
Um, has this resolved or normalized?
21:02
If it's a node, is it present
21:04
or is it present with progression?
21:07
Um, and so present really has like a,
21:10
does some heavy lifting here
21:11
because, you know, it can improve without resolving
21:15
or it can slightly increase in size
21:17
without really progressing.
21:19
And that all sort of just falls in that present category.
21:23
So here's what, you know, a, a table may look like for, um,
21:27
you know, your baseline
21:28
and your subsequent assessments where you're going
21:31
to document your sizes of your targets, the image numbers,
21:34
your sums of diameters,
21:35
and you're gonna do that at each time point
21:37
and measure those and, um, compare those.
21:39
And you're gonna look for decreased, uh,
21:41
percent decrease in the, um, sum, sum
21:44
of diameters from baseline or an increase from the Nader.
21:47
Um, these are non-applicable at baseline obviously,
21:50
because you're not calculating a change,
21:52
but you'll have these filled in,
21:53
in the subsequent time points.
21:55
Um, non-target lesions, again, it's qualitative.
21:58
You're just sort of talking about are they still there?
22:00
Are they, you know,
22:02
are they worse meeting progression or have they resolved?
22:05
And then presence or absence of new lesions.
22:08
And then again, other findings.
22:11
So just walk you through like an example here.
22:14
Um, this is a patient with metastatic colon cancer
22:16
with liver lesions.
22:17
These two studies on,
22:19
or these two images on top are from the baseline.
22:21
So you can see we have a lesion measuring 4.6 centimeters
22:24
and another one measuring 5.4 centimeters.
22:26
So our sum of diameters here is 10 centimeters on follow-up,
22:30
the lesions decrease in size to three three and two seven.
22:34
Um, and so those add up to six centimeters.
22:36
So when we calculate the, the percentage difference in, um,
22:41
in the sums of diameters,
22:42
we're getting a 40% decrease, right?
22:45
So that's gonna fall into this partial response category
22:47
of 30% or greater decrease in the sum of diameters
22:50
for baseline sum from baseline sum diameters.
22:53
So it seems pretty straightforward, right?
22:56
Of course, not all cases are straightforward like that,
22:59
but this is a, a good example when
23:00
you're sort of just learning.
23:03
Um, so targets are assessed
23:05
with these four categories that we've talked about.
23:07
Um, you know, I'll just review them again quickly.
23:11
Uh, complete response or crs disappearance of all lesions
23:15
and lymph nodes normalized.
23:17
Um, partial response is a 30% or more decrease.
23:21
Uh, progressive disease is a 20% or more increase, um,
23:25
or any new disease.
23:26
And then stable disease is really just like everything in
23:29
between PR and PD for your non targets.
23:33
We aren't going to be calculating these percentages
23:35
'cause we're not measuring things, right?
23:36
So the categories here are a little bit different.
23:38
We have a cr which is just like disappearance of e
23:41
of everything and normalized lymph nodes.
23:44
Um, PD is, uh, they use this term
23:47
of unequivocal progression, um, or, you know, new disease.
23:52
And so there's a little bit
23:53
of wiggle room here if something's like increased a little
23:56
bit and that's the judgment of the reader, like,
23:58
do you think that this is like unequivocal progression
24:01
or do you feel that it's equivocal?
24:04
Um, and so again, it's,
24:06
it's a qualitative assessment for you as a reader.
24:10
And then there's this category, instead of having PR
24:12
and sd, we have this non cr, non pd.
24:15
And so it's just basically a catchall of like anything
24:18
that falls in between these two.
24:20
So we have our assessments for targets,
24:23
we have our assessments for non-arts,
24:25
and then we have to sort of harmonize those
24:27
to give a global assessment.
24:29
And so you can see here you have whatever you've given your
24:33
target listed here,
24:34
whatever you've given your non-target listed here,
24:37
are there any new lesions?
24:38
And what's your overall response?
24:40
So an example
24:41
of this may be if your target lesions have gone away,
24:44
but your non-target disease is sort
24:46
of in this in-between category where it's not gone
24:49
but it hasn't progressed, you don't have any new lesions.
24:51
And so sort of the harmonization of this,
24:54
the targets carry a little bit more weight is gonna be, uh,
24:57
this is gonna be graded in overall partial response.
25:01
Um, you can see here that anything that has new lesions
25:04
or involves PD at any, you know, sort
25:07
of assessment is gonna result in pd.
25:13
So I mentioned this earlier when we're talking about partial
25:17
response, this is always gonna be
25:19
calculated in reference to the baseline.
25:22
Um, whereas progressive disease is gonna be in reference
25:25
to the Nader or the lowest point
25:27
or basically where the disease looked the best.
25:30
Um, and so this is kind
25:31
of a graphical representation of that.
25:33
So here's our baseline at the yellow arrow.
25:35
We can see over weeks that this disease has decreased,
25:39
this sum of diameters has really dropped
25:41
and we're down to like, you know,
25:42
a 40% improvement, which meets pr.
25:46
Um, this, you know, sort of stays where it is for the next,
25:49
uh, couple of time points.
25:50
And then we start to see disease grow and take off
25:53
and unfortunately hit the progressive disease.
25:57
So you can see that if you compared like this sum
26:00
of diameters to the baseline,
26:03
this is actually gonna look like a partial response, right?
26:06
But that would be incorrect
26:07
'cause you have to compare this to
26:09
where disease looked best.
26:10
And so, you know, disease improved
26:12
and then it started to, um, take off.
26:14
And then you do that calculation here.
26:17
So that's why you compare to the Nader.
26:19
Um, and here's like a pictorial example of that
26:22
where we have baseline, you know,
26:23
this large left lung lesion, which, uh, decreases in size
26:27
but then starts to progress by week 54.
26:32
So this is, you know, kind of, uh, you know,
26:36
what are the applications of these results
26:39
and what do we do with this res resus 1.1 categorization
26:43
and information that we get.
26:45
Um, so a lot of, uh, a lot
26:48
of the time we categorize objective responders
26:51
as patients who've resulted in a CR
26:53
or IPR, um, complete response or partial response,
26:56
and we put people in the stable disease
26:59
and progressive disease as non-responders.
27:02
Um, and so patients who progress, we can use this
27:05
to determine progression-free survival
27:07
or time to progression.
27:09
And for patients in the, um, you know, objective responders,
27:13
we can calculate overall response rates.
27:16
Um, so here's some examples of this.
27:18
Here's a time to progression.
27:20
You can see baseline, we've got, you know,
27:22
a significant improvement.
27:23
We meet pr and then we're at PR
27:27
until this like 54 week time point
27:30
where we've got this increase in, um, the sum
27:33
of diameters from the Nader.
27:34
So this is how we would calculate the time
27:37
to progression being 54 weeks from the time of like,
27:40
you know, improvement to the time
27:42
of the first documented progression.
27:46
Duration of response would be once we hit, uh, the PR
27:49
category, it's how long you stay there,
27:51
which we hope is either indefinite or ends in a cr.
27:54
But you know, in this case, unfortunately,
27:56
patient progressed again.
27:58
And so this is the same, the same case,
28:00
but the duration of response is this calculation here from
28:04
when the first time that we hit PR
28:06
to the first documented, um, pd.
28:12
So limitations of resist.
28:13
Uh, like I said, this can be really tricky if you don't
28:16
have targets, right?
28:18
If you're, if the majority
28:19
of your disease is non-measurable.
28:21
So things like ovarian cancer, um,
28:23
primary peritoneal disease, um, you know,
28:26
you may not have things that are easily trackable.
28:29
Um, other things like
28:31
that have poor measurement reproducibility.
28:33
So mesothelioma doesn't really grow in a
28:37
spherical mass like fashion.
28:39
It kind of grows in a rind, um, a rined morphology.
28:43
So we have different ways to measure that.
28:45
A modified, uh, system that we use,
28:48
masses that persist after therapy.
28:50
So we see this all the time with lymphoma, right?
28:53
Um, we can have lymph, no masses that we see by pet, uh,
28:57
undergo a complete metabolic response,
28:59
but we still have residual tissue there, right?
29:02
So, um, if you are just looking at size
29:05
and you're not really looking at the metabolic activity
29:08
of lymphoma, you may not be capturing like, you know,
29:11
your response as as accurately.
29:14
Um, so sometimes it's certain types
29:17
of disease like the three we just talked about,
29:19
but sometimes it's also the therapy.
29:21
Um, traditional chemotherapies are cytotoxic
29:25
and they act directly to kill cells, um,
29:28
to kill cancer cells.
29:30
Um, and so those should demonstrate responses
29:33
with a decrease in size.
29:35
But some of the newer targeted therapies,
29:37
particularly like the tyrosine kinase inhibitors
29:40
that target like vgf, E-G-F-R-A-L-K,
29:45
those are more cytostatic
29:46
and they're designed to sort of, sort of shut down cellular
29:50
proliferation and they're not really acting
29:52
with like direct cell killing.
29:54
Um, and so their responses may be less pronounced
29:59
and a little bit more of like disease stabilization
30:02
and more like modest decreases in size.
30:06
Um, so if you're really just only focused on size,
30:08
you might sort of be missing, um, these other
30:13
responses if you're, if you're dealing
30:14
with cytostatic drugs.
30:16
Um, so we'll go through some examples of these.
30:19
But, um, you know, gist, uh, metastatic gist is a,
30:22
a disease known to, um, when it's treated with Gleevec
30:26
to really have changes in density that may be more, um,
30:29
noticeable or, um, sort of pronounced than changes in size.
30:35
Um, you can have intratumoral hemorrhage with certain drugs,
30:39
uh, you know, as a part of their treatment response.
30:42
And you can imagine that may not lead
30:43
to a shrink in size of a tumor.
30:45
It might actually lead to a slight, uh, increase in size.
30:49
And then as we touched on
30:50
before, cavitations of lung lesions, cavitation is, um, uh,
30:54
an important feature that we see with like bevacizumab
30:57
or Avastin treatment, um, especially in in lung lesions.
31:03
So as I mentioned, mesothelioma has a nons
31:06
spherical growth pattern.
31:08
And so like how do you measure something
31:09
that's growing in like a hollow like cylinder sort of.
31:13
Um, and so we have a modified Resus 1.1,
31:17
which we basically like, uh, pick certain levels
31:21
and we measure in a perpendicular access to the chest wall,
31:25
um, and we do it at certain places
31:27
and we try to reproduce that at each time point.
31:32
As I mentioned with cavitation,
31:33
this is a metastatic colon cancer patient, um,
31:37
who's being treated with Avastin
31:38
and at baseline has a seven millimeter nodule.
31:41
Um, you can see at the six week follow up
31:43
that the lesions actually increased in its overall diameter
31:47
to 1.5 centimeters,
31:48
but there's, you know, it's mostly containing air
31:52
and there's less of this, uh, enhancing
31:55
or, you know, solid tumor tissue there.
31:58
So if you were, um, evaluating this with recess 1.1,
32:02
you're gonna call this a PD
32:04
because this is more doubled in,
32:05
more than doubled in size when in fact this is like a really
32:08
nice response that we're seeing here.
32:12
Um, like I mentioned with, uh, gist, that's naive
32:16
to any tyrosine kin kinase inhibitor.
32:19
So Imatinib or Gleevec is sort
32:21
of the most commonly used drug here.
32:23
Density is really important
32:24
because part of the treatment response here is OID
32:27
degeneration, um, hemorrhage necrosis, sort
32:30
of liquefaction of the tumor.
32:32
Um, and so what we notice with these lesions are is
32:36
that they dramatically drop in density.
32:38
Um, they might actually appear larger
32:41
or easier to see, um, especially in the liver.
32:44
And so you really wanna be careful
32:46
that you're not misinterpreting those changes
32:49
for progressive disease.
32:50
Um, you can use PET ct, uh, FDG PET CT in cases where it's,
32:55
you know, not really clear,
32:56
but treated lesions should really be NFDG negative if
32:59
they're, you know, filled with all of this, uh, material
33:02
and not enhancing tumor.
33:05
So here's some, uh, examples of this.
33:07
This is metastatic just to the liver, oops, sorry.
33:11
Where you can see we have, um,
33:13
this lesion in the right low measuring 2.8 centimeters
33:17
and then the left lo measuring 1.7 centimeters on baseline,
33:20
so a sum of diameters of 4.5 centimeters.
33:23
Um, on follow-up you can see that this is increased
33:26
to three nine and two nine here, um, which would be,
33:30
you know, a 6.8 centimeters sum of diameters.
33:32
And so this is gonna be a 50% increase, which would classify
33:37
as a progressive disease.
33:38
But if you look more closely, the density
33:41
of these lesions are, you know, sort of slightly hypo dense
33:45
or hypo enhancing to background liver on the baseline.
33:48
And then when you look on the follow-up, the,
33:50
the density is really dropped here.
33:52
We definitely have like a significant fluid component
33:55
and there is still some enhancing tumor here,
33:58
but the amount of tumor tissue compared
34:00
to baseline has decreased.
34:01
You can sort of see the same thing going on in
34:03
this lesion in the left lobe.
34:04
There's now like a significant
34:06
component of it that's not tumor.
34:08
Um, and these also have intratumoral hemorrhage
34:11
and so you sort of don't know is what I'm seeing blood
34:14
or tumor or OID degeneration.
34:16
So here's um, MR post contrast of, uh,
34:21
of these, of this patient.
34:23
Um, this size is pre and post contrast.
34:25
And so you can see that this is T one hyperintense material
34:27
in here, probably blood
34:29
or pro nastious material, um, um, which is not enhancing.
34:32
So in fact, this is really an excellent response to therapy.
34:36
So you can see where reist like doesn't really cut it
34:39
for assessing or capturing response
34:42
of these drugs in these particular malignancies.
34:47
Um, so in response to that, there's been development
34:50
of the choi and modified CHO criteria.
34:53
Um, it's not really the topic for today's,
34:55
so I'm not gonna dive too much into it,
34:57
but I just wanted to make you guys aware of it.
34:59
But you can see it uses a similar response, um, as, uh,
35:03
categories of CRPR, uh, SD and pd.
35:07
Um, and there is some certain, you know, overlap
35:09
of like a CRS disappearance
35:11
of all lesions with no new lesions.
35:13
But, um, there's sort of different thresholds
35:16
for the changes in size.
35:18
And there's also this allowance for decreases in, um,
35:21
in tumor attenuation, um, measured in hounde units.
35:25
So you really need CT for these.
35:27
Um, they also have some clinical criteria
35:31
as well incorporated.
35:32
But, um, yeah, one, one thing you also wanna look out
35:37
for in these is these can develop intratumoral nodules.
35:41
Um, you know, they can develop or increase in size.
35:44
And so you can imagine if the overall size
35:46
of the lesion isn't changing, you could sort
35:49
of miss a progression if you're not
35:50
looking for these nodules.
35:53
These are more tied to changes in character
35:55
of the tumor rather than just size.
35:57
So, um, here's an example of this.
35:59
This is like a post-treatment metastatic gist to liver,
36:02
and you can see these like very low density cystic looking,
36:07
um, lesions, which are, you know, just treated disease.
36:10
And then on follow-up you can see the development
36:12
of these little intratumoral nodules
36:14
that the arrows are pointing at.
36:16
Um, and then at a subsequent time point they've like
36:19
significantly increased.
36:20
Um, and we've confirmed with pet CT over here
36:23
that these are in fact active and viable tumor.
36:26
So, um, you know, Reeses really focuses heavily on size,
36:31
but size isn't always the whole story.
36:34
So this is a really, I think, an important concept
36:37
to integrate at the workstation, right?
36:39
Um, we can all sit there and look at, at lesions
36:42
and say, you know, same, bigger, smaller, no significant,
36:45
you know, changes or whatever,
36:47
but you really have to go beyond that
36:48
and also look at the character of, of the lesions
36:52
and you know, especially when you're dealing
36:54
with certain histologies and,
36:56
and certain drugs that are being used.
37:00
Here's another example.
37:01
This is metastatic renal cell carcinoma.
37:03
This patient's on sorafenib, um,
37:06
which is a tyrosine kinase inhibitor.
37:07
A little clue is anything
37:08
that ends in an IB is probably a tyrosine kinase
37:11
or kinase inhibitor.
37:12
And one of these like targeted, um, psychos static drugs.
37:17
Uh, but on first glance you see on your baseline we've got
37:21
some, you know, nasty looking hypo enhancing lesions
37:24
with a hyper enhancing rim.
37:27
Um, you can see several of these
37:29
and then on follow up, I think, you know,
37:31
your first instinct might say like, wow,
37:33
there's so many more lesions.
37:35
This is, this is progression, right?
37:37
But when you actually look at the character
37:39
of these lesions, you know, this dominant one here in the
37:41
left lobe, we've lost our hyper enhancing rim.
37:44
The density's really decreased.
37:45
There is still like an internal septation,
37:47
but there's not that same enhancing, um,
37:50
hypo enhancing tumor in there.
37:53
Um, and then, you know, we sort of see same story going on
37:56
with this other segment four lesion.
37:58
And you know, this one here on the
38:00
right that's partially visualized.
38:01
And then when you look at these ones along the periphery
38:04
of the right lobe, when you, in, in retrospect, you can see
38:07
that these are actually here,
38:08
but they're just sort of iso to slightly hyper
38:11
to slightly hypo enhancing on the baseline.
38:14
And so you are appreciating and seeing more lesions.
38:18
But the reason for that is because the density has dropped.
38:20
And so this is actually a response in
38:23
previously occult lesions.
38:25
So this is another, you know, thing to just be aware of,
38:28
especially at the workstation is, you know,
38:31
are you actually seeing new lesions
38:33
or are is this response in lesions
38:35
that were difficult to see before?
38:40
So again, this is that table I showed you
38:42
before with the various assessment, um, response criteria
38:46
and mass is one that's used in renal cell carcinoma
38:49
and it doesn't use the same categories as the rest of them.
38:52
It has more of like a favorable response, uh,
38:55
an intermediate response
38:56
and an unfavorable response with, you know,
38:59
different thresholds, uh, for size,
39:01
but it also accounts for decreased attenuation.
39:04
So just another one to sort of be on the radar.
39:08
Another class of drugs that we, um,
39:10
are using in clinical trials
39:12
and in clinical practice are immune checkpoint, respo, uh,
39:15
immune checkpoint inhibitors.
39:17
Um, and these have really, um, sort of different, uh,
39:22
and can be very atypical response patterns, um,
39:25
particularly early in the course of treatment.
39:28
Um, and so we've created, you know,
39:30
a separate response criteria to address tumors
39:33
that are treated with these drugs.
39:34
And so you can see there's different thresholds for the, um,
39:37
changes in size.
39:39
These are done in bi-directional measurements.
39:41
And the real key differentiation here is that we require,
39:46
um, that response can mimic pd
39:49
that's called pseudoprogression.
39:50
I'll show you some examples of this in a minute.
39:53
Um, and that we need reassessment on scans
39:55
that are at least four weeks apart to really sort
39:57
of be certain about what we're seeing.
40:00
So I'll show you just quickly, there's four patterns
40:03
that we've observed with immune
40:04
checkpoint re um, inhibitors.
40:06
And you know, one is what we expect to see with, you know,
40:09
most other drugs is a decrease in size
40:12
or, um, you know, a resolution of a finding.
40:15
So this chest wall lesion in a malignant melanoma has, um,
40:20
you know, certainly decreased in size here over time.
40:23
Uh, another pattern we can see is long periods
40:26
of just basically stabilization.
40:29
Sometimes this is followed by, uh,
40:31
an eventual decline in the term tumor burden.
40:34
Um, this is another metastatic melanoma case.
40:39
Um, and then, uh, patterns three
40:41
and four are ones showing pseudoprogression.
40:43
So here you can see at again, metastatic melanoma.
40:47
We've got this axillary lymph node,
40:48
which at the first time point
40:50
significantly increases in size.
40:51
This is like more than doubled.
40:53
This is probably four times its original size.
40:56
Um, I don't know if you can appreciate here,
40:58
there's a little bit of a drop in density
40:59
and a slight decrease in size at time 0.3.
41:02
And then we have like kind
41:04
of a dramatic decrease in size shrinkage to almost,
41:07
you know, near complete response by time 0.6.
41:11
Um, and so what this is is a delayed tumor response, right?
41:15
We have a known site of disease
41:17
that gets worse before it gets better.
41:20
Um, this is thought to reflect like there's,
41:23
there's two things that we believe this represents.
41:27
So number one is that it takes time
41:29
to train the immune system, um,
41:31
to fight these particular malignancies
41:34
using these particular drugs.
41:36
And so there is actually true growth that occurs
41:39
before the immune killing sort of kicks in
41:41
and takes care of disease.
41:43
The other thing is when you have immune infiltration
41:45
of sites of disease, you can have some edema
41:47
and some swelling that will make lesions, you know,
41:49
get a little bit bigger and look worse
41:51
before they, um, start to improve and, and respond.
41:54
We have biopsies showing both of these scenarios.
41:58
Um, so here's another one.
42:00
This is again, metastatic melanoma to the ally.
42:02
You can see it definitely gets worse.
42:04
We've got a drop in density, which doesn't always happen,
42:06
but in this case it does.
42:08
And then we've got an eventual decline in the size.
42:13
Uh, this is a really interesting case.
42:14
So we've got metastatic melanoma to the muscles
42:17
and soft tissues of the lower extremities on both sides.
42:20
Um, and you can see at time 0.1,
42:22
we definitely have an increase in, you know,
42:24
abnormal tissue in, on both sides,
42:26
but dramatically so on the right.
42:28
So by recess you're gonna call this, um, progression even
42:33
by choi criteria or mass criteria.
42:35
This has not demonstrated a significant decrease in density.
42:39
In fact, areas are looking more dense and more enhancing.
42:41
So you're gonna call progression here as well,
42:44
um, with those criteria.
42:45
And then we can see at time 0.3 everything is gone,
42:48
which is just sort of incredible.
42:50
Um, so that's why sort of the extra time points, um,
42:55
especially early on in treatment are required
42:57
to really determine what sort of response is happening.
43:01
Here's another one of Hodgkin lymphoma.
43:03
You can see there's quite a bit of disease at baseline.
43:05
I'll draw your attention to this dominant mesenteric mass,
43:08
which, um, you know, over time points two
43:11
and three continues to get bigger.
43:13
Um, we've got some sort
43:14
of mixed response going on in the chest.
43:16
Some of these lesions are looking a little bit better.
43:19
Um, but by, you know, time 0.4
43:21
and time 0.5, we've got like a complete response.
43:24
Um, so this can be really, really tricky.
43:27
Pseudoprogression, I don't want you
43:28
to walk away thinking this is like the most common thing
43:30
that we see, but it's um, it's documented in like, you know,
43:34
three to 10% of cases.
43:36
So most of the time when you see progression,
43:38
it's gonna be true progression,
43:39
but if you're in the first like 12 to 15 weeks of treatment,
43:42
you really should consider pseudoprogression as well.
43:45
This is just a graphical representation of the two, um,
43:48
things we talked about, actual tumor growth before response
43:52
and you know, just immune infiltration
43:53
and swelling before response.
43:56
Um, the fourth and final pattern is where we see
43:58
what we think is new disease.
44:00
And this is really just pseudoprogression in
44:02
previous like micro metastases that just we weren't able
44:06
to visualize yet, but it's the same sort of scenario.
44:09
Here's some more examples of, um, pseudoprogression.
44:12
So we can see normal looking bone.
44:14
Here we are very early week eight, uh,
44:17
we see a new lytic lesion, which then by week 17 has healed.
44:21
Um, we see no lymphadenopathy here,
44:24
new lymphadenopathy in the pelvis,
44:25
and then an improvement, um, normal looking bone mixed, uh,
44:30
or mostly lytic, you know, nasty looking disease here,
44:34
which then eventually heals.
44:35
So the pseudoprogression is really something to be aware
44:38
of early on in treatment.
44:40
So again, the response pattern that we use to determine, um,
44:45
you know, if a drug is working
44:47
or if disease is progressing depends on both what kind
44:51
of disease it is, but also what kind of drugs we're using.
44:54
So those are things I like
44:55
to know when I'm reading cancer cases, you know,
44:57
what's the histology, what drug are they on,
44:59
and how long they've been on it
45:01
because it can sort of tell you which principles should we
45:03
be using to assess response
45:05
and what sort of atypical pattern should we be expecting.
45:09
Um, this is a really great resource.
45:11
This is like one of my homepage
45:12
that I use the National Cancer Institute,
45:15
um, drug dictionary.
45:16
You can like search any drug
45:18
'cause it's impossible to memorize all of them.
45:20
Um, and it will tell you like a very sort of succinct, um,
45:24
you know, mechanism of action that can clue you into,
45:27
you know, what, what type of drug
45:29
and what category it falls in, which will help you determine
45:31
what kind of response you're looking for.
45:34
Here are my references and I'm happy to take any questions.
45:38
Um, I know this was a very dense topic, so, uh,
45:41
appreciate all of your attention and interest.
45:47
Well thank you so much Dr.
45:48
Macintosh for that awesome lecture.
45:52
We will open the floor for some questions,
45:54
so if you've got them, go ahead
45:56
and stick that in the q and a box.
46:00
Oh, let's see, q and a, sorry.
46:02
No worries. Role of
46:04
and brain tumors post radiosurgery response.
46:07
So yeah, sorry, I did not mention this,
46:09
but, um, we have different response criteria for,
46:12
for neuro-oncology.
46:14
So recess isn't really used uh, for, for brain tumors.
46:18
This is mostly recess is used for solid tumors, um,
46:21
and mostly sort of in the, in the body.
46:24
Um, you know, outside of neuro
46:29
are you able to change target lesions and recess criteria?
46:33
Say post-treatment, there is new disease for follow-up.
46:36
So no recess is really inflexible.
46:38
Um, which is why it's very important
46:40
to get the baseline right.
46:42
Um, you aren't able to change targets, you sort
46:45
of have to follow them forever.
46:47
Um, and that's why you also wanna make sure
46:49
that you're catching all disease
46:51
and using them as um, you know, either targets
46:55
or non-arts because you wanna be able to follow what happens
46:59
and track what happens with the non-arts.
47:01
And then any new disease,
47:03
of course you give it a categorization of like new lesion,
47:06
that's sort of like a third category.
47:10
Alright, when target lesions decrease
47:12
or are completely gone,
47:14
but non-target lesions appear,
47:17
is it considered a progression?
47:19
So anything that appears would not be a non-target,
47:23
that would be considered a new lesion.
47:25
And yes, that would be progression.
47:27
Anytime there's new, um, disease is progression.
47:32
Let's see, for lymph node measurement,
47:33
do you measure the short axis
47:35
or the long axis to determine the sum of diameters?
47:39
Um, so for lymph nodes, you uh, you measure
47:42
and report the short axis, um,
47:44
and that's what gets calculated in your sum of diameters.
47:49
Alright, looks like it takes familiarity
47:51
and experience to get used to how each
47:53
and every tumor behaves and respond.
47:55
Do you have a table for patterns based on your personal case
47:58
experience to make it easy to remember
48:00
and categorize new patient cases?
48:03
Um, you're absolutely right.
48:05
Um, it does take lots of familiarity
48:08
and experience and practice.
48:10
Um, you know,
48:12
and I would say it's actually even more important in
48:14
clinical practice than it is.
48:15
Um, you know, in the clinical trials they basically tell you
48:18
what to use, um,
48:20
and you know, that's determined
48:21
by whoever's designing the clinical trial.
48:23
And so, um,
48:24
sometimes they actually have you use more than one response
48:27
criteria and you're sort of doing different measurements
48:29
because they're not sure which one is gonna categorize it,
48:32
um, categorize it best.
48:35
But, um, yeah, I sort of, I just think about what,
48:40
what disease looks like, um, how it grows,
48:44
how it responds, um,
48:46
and that might be different based on which type of,
48:49
you know, drug is being used to treat it.
48:52
So I don't,
48:53
but that would be a really good idea for a publication
48:55
to sort of, um, try to categorize those and,
48:59
and figure out, you know, a workflow
49:02
or an algorithm of like what to be thinking about
49:04
with different cancers and different drugs.
49:07
Thanks for the idea.
49:10
Um, is there any problem if I do like a pseudo reist,
49:15
sometimes we don't have the first study of the patient
49:17
to check the target lesions.
49:19
How can we report that?
49:21
So reist is like a formal reist read is only really
49:26
required in the setting of a clinical trial where you would,
49:29
you would have to have all of those things.
49:31
Um, sometimes trials give like an allowance
49:34
for like if a baseline is missing then you know,
49:36
this is exactly how you would document it.
49:39
Um, but in clinical practice, if you don't have a baseline,
49:44
I mean there's not really much you can do.
49:46
Uh, you can only see what you say or, or say
49:50
or talk about what you see.
49:52
Um, and so you can certainly compare subsequent studies
49:56
to the earliest one that you have available.
49:58
But, um, I wouldn't,
50:00
I wouldn't be doing anything formal about like
50:02
targets or non-arts.
50:03
It's just sort of like a clinical read would be very,
50:07
you know, you can certainly measure things
50:08
and talk about things, but I wouldn't be giving like a,
50:11
a formal recess report on that.
50:12
I would just sort of be like your usual clinical report.
50:16
Okay. Um, cervical chain nodes are also short axis.
50:21
Um, yes, the nodes are measured the
50:23
same no matter where they are.
50:24
And like I said, it's important to remember that the, um,
50:28
lymph nodes are globally one organ
50:30
and so you can only choose two of those
50:32
with reist if you have a lymph node predominant
50:35
disease like lymphoma.
50:37
We don't use reist in, in lymphoma at all.
50:39
We have a separate one called Luo, um,
50:42
which is very pet heavy,
50:43
but there is like, you know, CT only criteria as well
50:46
and those are actually measured in long and short axis
50:49
and we use both of those in a calculation
50:52
of a sum of diameters.
50:53
So lymphoma is a totally different story.
50:57
Alright, how would you differentiate
50:58
and report a visually new lesion
51:00
that's pseudoprogression versus true progression?
51:03
So, um, in trials you basically would report it
51:07
as a new lesion, but you can flag it as something
51:10
that you think is pseudoprogression
51:11
and you can sort of look at the subsequent time point
51:14
and you know, you might need that subsequent, you need
51:16
that subsequent time point to determine if it's progression,
51:20
uh, versus pseudoprogression for a clinical read.
51:23
Um, I will, you know, an example of a read
51:26
that I would give is I would say there's slight in,
51:29
you know, there's increase in size
51:30
of the right liver lesion.
51:33
Um, you know, given the
51:36
short time intervals since initiation of treatment,
51:39
this could represent progression versus pseudoprogression
51:43
recommend a follow-up exam in no less than four weeks.
51:47
That's sort of how I would phrase it, is that you have
51:49
to list both in the differential if you, you know,
51:52
if both are in the differential
51:53
and then request a subsequent time point.
51:55
And then that's sort of where you,
51:57
you the pseudoprogression versus true progression is always
52:00
something that's made in retrospect.
52:01
You can't tell at the time point times
52:03
that I think more about pseudoprogression are when I see a
52:07
mixed response if, if you know, something's getting worse,
52:10
but then I also see things that are getting better that sort
52:12
of makes me think more about
52:14
pseudoprogression than true progression.
52:17
Um, when the size of the lesion increases,
52:20
how can we suggest pseudoprogression
52:22
rather than progression?
52:23
Oh God, I just answered that one.
52:25
Um, you can't always, a lot of times you have
52:27
to give both in the differential,
52:28
but again, if there's a mixed response, it, you know,
52:31
might make me lean one way a little bit more than another.
52:34
All right. PD assessed based on Nader,
52:37
but what if we do not have the Nader any surrogate?
52:40
Basically you have to just work with what you have
52:42
and you figure out, you know,
52:44
however long the patient's been on this particular drug
52:46
or treatment regimen, what is the time point
52:48
where their disease look best?
52:50
And then you have to sort of base it on that.
52:54
Is there an automated program
52:55
for calculating status in reus 1.1?
52:59
Um, there are, and actually quite a few PAC systems, um,
53:03
have, uh, you know, programs built right in to be able
53:06
to do this, you just have to sort of like,
53:08
you do the measurements and the um, the numbers get imported
53:11
and also the calculations of the changes.
53:14
Um, and most of the clinical trial, uh,
53:18
like there are programs like Mint is one, um, that's used.
53:22
Biore is another that, um, you basically do the measurements
53:27
and they get, uh, automatically inputted
53:29
and managed, um, like that.
53:31
So yeah, there is automation,
53:32
which makes things a lot easier.
53:35
Alright, new brain metastasis is always pd.
53:39
Yes, any new site of disease
53:40
and, um, sometimes that happens where, you know,
53:44
a trial may only have chest, abdomen, pelvis imaging
53:47
and then suddenly at a time point you get a brain Mr thrown
53:51
in there that has like a new lesion, especially
53:53
with something like lung cancer.
53:55
And that would trigger a pd even if it's like you can sort
53:58
of assume that it's a new lesion even if you don't have, um,
54:02
priors based on, you know, clinical presentation
54:04
or, or whatever.
54:07
Um, okay. Do you use Resus in breast cancer?
54:11
So yes.
54:13
Resus can be used in, um, in, in metastatic breast cancer
54:16
that requires chemotherapy.
54:18
Um, we're starting to see, you know,
54:20
there's like different drugs
54:21
that are being used in breast cancer
54:22
and even those immune checkpoint inhibitors are being used.
54:25
So it, it does also depend on the particular drug.
54:28
But yes, you can use Resus 1.1 in breast cancer. Okay.
54:33
I've had cases where pseudoprogression progress for one
54:36
to three years, would these lesions be called
54:39
pseudoprogression versus progression for the one
54:41
to three years of scans?
54:43
So probably not at that point.
54:45
I really think about pseudoprogression in the first
54:47
12 to 15 weeks.
54:49
It has been documented out to like, you know,
54:51
40 or 50 weeks.
54:53
Um, but I think that's really the
54:54
exception rather than the rule.
54:56
Um, if something is progressing at one to three years,
55:00
it's probably true progression
55:02
because the disease has either mutated
55:04
or for whatever reason is not
55:05
responding to the drug anymore.
55:07
So at that time point, I think it would be safe to,
55:10
you know, definitely call that true progression.
55:13
What is a Nader?
55:15
So a nader is just the word that we use
55:17
to describe the time point where disease looks the best
55:21
or has the greatest response.
55:23
Um, and so that might be the first time point
55:27
or it might take several time points to get there.
55:29
Um, if you have progression right away, uh,
55:31
like at your first time point,
55:32
then you don't really have a Nader
55:34
because you just have your baseline.
55:37
Alright. Non-target bone lesions, any new is pd? Yes.
55:42
Any new lesion, um, is pd, no, nothing
55:46
that's new is gonna be classified
55:48
as a target or a non-target.
55:49
It's just simply going to be called a new lesion.
55:55
You got 'em all? Alright,
55:58
that was excellent. Thank
56:01
You guys. And those are some
56:02
really great questions.
56:03
There's always interest in pseudoprogression
56:06
and sort of how to, how to parse that out.
56:10
It's, um, it's a, a really tricky thing, right?
56:12
Because it looks exactly like progression
56:14
and it, it feels funny to put in your differential.
56:16
Like this could be pseudoprogression, which is a response,
56:20
you know, gonna eventually be a response
56:21
or this could be progression.
56:23
And so it's like they're sort of opposites
56:24
and it, it feels funny to put those in your differential,
56:27
but, um, with these drugs they just, they can be very
56:31
challenging and, uh, have unexpected, you know,
56:35
response patterns that um, you just really need more time
56:38
to figure out what's going on.
56:40
Oh, a couple more questions came in.
56:42
Oh, if you wanna go for it. Yeah.
56:45
If we have a target lesion
56:46
with cavitation in follow-up study,
56:48
should we still measure it in the long axis,
56:50
include it in the sum of diameters,
56:51
and just additionally report the change of morphology.
56:54
So yes, in a 1.1 formal read in a clinical trial,
56:59
you would still measure it.
57:01
Um, and you can certainly leave comments, um,
57:05
about the change in morphology.
57:07
In a clinical read, I would like absolutely lead
57:10
with the change in morphology
57:12
and I would, in my impression call it a response,
57:15
even if the size is unchanged
57:17
or even slightly bigger, uh, in a patient with lung cancer
57:21
and brain metastases on the baseline exam, non-target,
57:25
which disappeared by the second
57:27
and third follow-up, will the reappearance
57:30
of the brain lesion by the fourth be classified
57:32
as pd if target lesions are pr?
57:35
So this can be trial specific.
57:37
Um, if you feel
57:39
that the lesion has like fully disappeared,
57:43
you can't detect it on, you know, any, any part
57:47
of your imaging, then you know,
57:49
the reappearance would be considered, like it would be,
57:52
you would have to document it as a new lesion
57:54
because once you've documented a target lesion as resolving,
57:58
um, you can't really resurrect it or bring it back.
58:00
So it would have to be classified as new lesions.
58:04
Um, sometimes for like pet studies, uh, pet clinical trials,
58:09
if you have something that like the metabolic
58:12
avidity resolves,
58:14
but then it that comes back, that's more likely
58:17
to be classified as like a, a local recurrence of a target.
58:21
Um, and,
58:22
and not like a new lesion, it's just that, you know,
58:25
the avidity got so low that we weren't really able
58:27
to appreciate it, um, you know,
58:29
with micrometastatic disease or whatever.
58:31
So it's kind of trial specific.
58:34
Um, and it could, it could go either way,
58:37
but if you have cleared a target
58:39
or even non-target lesion, if you've said
58:41
that it's completely resolved
58:42
and you truly believe that, then
58:45
that would be considered new disease.
58:49
Let's see. Do you have any experience
58:51
of post radiosurgery changes on CT in hepatocellular cancer?
58:56
Like change in enhancement patterns?
58:58
Yeah, that's a little bit outside of the scope
59:00
of this lecture,
59:01
but um, yes, you can certainly have like, you know,
59:06
changes in the enhancement patterns
59:08
of hepatocellular carcinomas after radiation
59:11
and changes of like the surrounding parenchyma
59:13
and changes that do suggest recurrence.
59:16
Um, particularly like, you know, new
59:18
or increasing areas of, um, nodular
59:21
or peripheral enhancement like at the, at the margins
59:24
of the lesion or the treatment field.
59:27
Alright. Can you repeat the time you use to guide yourself,
59:31
uh, to think it might be pseudoprogression versus
59:34
progression since the SAR of treatment?
59:35
Yeah, it's usually in the first 12 to 15 weeks is
59:38
where pseudoprogression is most commonly seen.
59:42
Um, you know, if we were at like 16 or 17 weeks
59:45
and the patient's like,
59:47
and another part of progression in pseudoprogression is also
59:49
how is the patient doing?
59:51
Um, sometimes we have oncologists come in
59:53
and they say like, man, this, this study was read
59:56
as like worsening, but the patient's doing great.
59:58
They feel awesome. You know, that might sort of also that
60:03
that can sort of help figure out, okay,
60:05
should they stay the course, should they keep doing the
60:07
treatment and you know, re-image
60:08
and, you know, give them the benefit of the doubt
60:10
that this could be pseudoprogression.
60:12
If that's the case at like, you know, 16, 17 weeks,
60:14
I'll still certainly consider that it's not like a hard
60:17
and fast at 12 to 15,
60:18
but that's sort
60:19
of the most common time period in which this occurs.
60:24
Um, can we consider the volume
60:25
of a lesion rather than the short axis?
60:27
So yeah, a lot.
60:28
There's actually like, you know, many people that feel
60:31
that volume of lesions is uh, superior to, um, you know,
60:36
looking at unidimensional
60:37
or bi dimensional measurements, um, that it's more,
60:41
you know, able to capture changes a little bit better.
60:44
Um, that's not what's used in Resus 1.1.
60:47
And a big part of that I think is just
60:49
because what, what is available to us
60:51
as radiologists, right?
60:53
Not everybody has like vol volume tree available to them.
60:57
And we can also see differences across platforms, you know,
61:00
between volume tree,
61:01
but again, like, you know, by dimensional, uh,
61:05
or manual measurements are certainly not, uh,
61:08
always reproducible.
61:09
We have inter observer and inter observer variability.
61:12
So, um, no system is perfect.
61:15
Some people do really like volume
61:17
and there are some assessment criteria
61:18
that use tumor volumes,
61:19
but for resis 1.1, it's really just, uh, a manual
61:25
single dimension measurement.
61:29
Okay. I think that was all of 'em. I
61:31
Think, I think you got it all.
61:34
Thank you so much.
61:36
Yeah, thank you guys. Thanks for your attention.
61:38
Yeah, thanks everyone for asking such great questions
61:40
and for signing on to today's NOOM conference.
61:44
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61:46
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61:47
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61:48
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61:53
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61:54
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61:57
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61:59
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62:03
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62:05
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62:07
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62:08
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Director, Oncologic Imaging; Assistant Professor, Radiology
University of Massachusetts Medical School / Memorial Health Care
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