Cellular determinants of anti-tumor immunity in human cancers

Name: Cellular determinants of anti-tumor immunity in human cancers
Uploaded: 2025-06-11T11:27:31.2666667Z
Duration: 10 min
Description: Physician-scientist Benjamin Lu, MD, PhD, presents on cellular determinants of anti-tumor immunity in human cancers

June 11, 2025

Physician-scientist Benjamin Lu, MD, PhD, presents on cellular determinants of anti-tumor immunity in human cancers

About the speakers

Benjamin Y. Lu, MD, PhD
Assistant Professor of Medicine (Medical Oncology/Hematology); Kathryn Louloudis Scholar in Cancer Research, Medical Oncology and Hematology

Information

ID: 13221
To Cite: DCA Citation Guide

Download Transcript

00:00To do is just briefly
00:02go over kind of our
00:03approach towards
00:05studying cancer immunology in humans.
00:07And my particular interest moving
00:09forward is going to be
00:10in studying immune and cancer
00:12cell interactions and how
00:14they shape
00:15anti tumor immunity overall.
00:18But we do this in
00:21by by first taking a
00:22look at
00:24patient specimens, clinical questions, relevant
00:27clinical questions,
00:28and then using
00:29techniques to try and understand
00:31fundamental aspects of human immunology.
00:33And so to do this,
00:34we first have simple questions
00:36using high dimensional techniques such
00:38as single cell sequencing.
00:41For example, what who are
00:42we looking at? What is
00:43the transcriptional,
00:45heterogeneity that is present within
00:47tumors and immune cells?
00:49What is the function and
00:50what is the interaction that's
00:52going? And in the case
00:53of t cells, which is
00:54where our biases
00:56lies, we then ask, you
00:57know, where else can we
00:58trace these t cells to?
01:00And,
01:02how are the microenvironment really
01:04influencing,
01:05Timur and Mindy? And, ultimately,
01:08with
01:09the the phenotypes that we
01:10identify and
01:12these fundamental
01:13mechanisms that we identify, how
01:15can we leverage this back
01:16into the clinic for clinical
01:18intervention?
01:19And so, one vignette I'd
01:21like to just bring up
01:22that's published that I'll briefly
01:23go over, and this is
01:24actually, a project I was
01:26co mentored with doctor Kluger
01:27and funded by the Skinspor,
01:30that we did in the
01:31extracranial
01:32setting with patients with melanoma.
01:34We first identified
01:35that
01:36there's
01:38a
01:39subpopulation
01:40of CD8 T cells that
01:41is tumor antigen specific,
01:44but is actually highly resembles
01:47recently described,
01:48CD8 regulatory T cells, and
01:49so it dampens antitumor immunity.
01:53We were able to trace
01:54these out into the blood
01:56and found that the levels
01:57that we find in the
01:58blood correlate with those that
01:59are in the tumor.
02:01And as mentioned, they impair
02:03antitumor immunity, and what we've
02:05found was that it does
02:06so by targeting other antigen
02:08specific t cells
02:10and that ultimately this results
02:12in
02:13poor patient outcomes.
02:16But the second vignette that
02:17I'd like to focus on
02:18really stems from our ability
02:19to leverage kind of
02:22fundamental aspects that we've learned
02:24through the years
02:26and to bring them back
02:27into the clinic. And so,
02:28this is ongoing work that,
02:30is unpublished,
02:31but,
02:32that
02:34we are working
02:35on right now in patients
02:37with glioblastoma.
02:38So
02:39in patients with glioblastoma,
02:40immune checkpoints really have not
02:42worked well. Anti p d
02:44one regimens have failed to
02:45improve survival for patients,
02:47in multiple
02:48phase three trials. Hypothesized mechanisms
02:51of failure include
02:53activation of regulatory t cells,
02:54so the suppressive t cells,
02:56in addition to changes in
02:58the cancer cell plasticity and
03:00glioblastoma cancer cells,
03:02among many other regimens. But,
03:04a couple years back, we
03:06leveraged,
03:07this kind of institutional expertise
03:09in regulatory t cell biology
03:10and identified,
03:12alternative,
03:14coin receptor called TIGIT,
03:16which we understand to be,
03:18unlike PD one, more important
03:20for stabilizing the suppressive function
03:23of regulatory T cells.
03:24This is work that was
03:26done out of the Haffler
03:27lab that suggests that,
03:29TIGIT expressing regulatory T cells
03:31are more suppressive than TIGIT
03:33negative, not nonsuppressing T cells,
03:35and that when placed into
03:36pro inflammatory environments,
03:38TIGIT engagement, TIGIT signaling
03:41through CD one five five,
03:43helps stabilize the suppressive phenotype.
03:46Now we also know that,
03:49TIGIT is highly expressed in
03:50addition to its binding partners,
03:51highly expressed in glioblastoma,
03:55unlike in multiple sclerosis, which
03:57is a pro inflammatory
03:59condition in the CNS.
04:02And that therapeutically targeting both
04:04TIGA and PD-one
04:05in humans and also
04:08in preclinical models,
04:10helps improve pro inflammatory
04:12conditions.
04:13And so,
04:14this led to the institutional
04:16initiated trial,
04:17led by doctor Amearl and
04:19close collaboration with doctor Malinturno,
04:22and since taken over by
04:24doctor Kurz,
04:25for this IIT that, is
04:26investigating the combination of anti
04:28PD one and anti TIGIT
04:30in patients with recurrent glioblastoma.
04:32And this is a two
04:33part trial. The first part
04:34was a safety lead in.
04:35But the second part, right,
04:37is a perioperative condition where
04:39patients get
04:40one of four treatments prior
04:42to going to surgery, so
04:44either antitigid alone, anti PD-one
04:46alone, the combination, or placebo
04:48followed by combination afterwards. And
04:50this really allows for us
04:52to collect
04:53tissue
04:54specimens to try and understand
04:56aspects of
04:57tumor immunity.
04:59And so we've designed
05:02translational studies to try and
05:04really
05:05deeply
05:06analyze what
05:08are the perturbations that occur
05:10following these perioperative
05:12treatments.
05:13And, the the trial has
05:14just
05:15concluded
05:17accrual, so a lot of
05:18these studies are ongoing. Has
05:28referenced earlier is being run-in
05:30close collaboration with Rong Fan
05:31and Yang Liu, in addition
05:33to Marcello Distasio, who's a
05:34neuropathologist.
05:36But we do have some
05:37preliminary data that does give
05:39us, some optimism that, you
05:41know, biological activity is occurring
05:43in these patients.
05:45And these include that at
05:46very early time points, we've
05:48observed a
05:49shift towards effector phenotypes,
05:51effector t cell phenotypes in
05:53circulating populations in the blood.
05:55And so what I'm showing
05:56on the bottom are results
05:57from flow cytometry data from
05:59our safety reading
06:00that suggests at day five,
06:02as early as day five,
06:03we see a shift from,
06:06more naive,
06:07or memory populations towards effector
06:09populations.
06:10This is also reflected in
06:12their ability to secrete cytotoxic
06:14th one cytokines.
06:15This occurs from from both
06:16CD8s and CD4s.
06:18And based off of our
06:19preclinical,
06:21hypotheses,
06:21TIGIT would,
06:23differentially impact,
06:25regulatory T cell phenotype. We
06:27also do see shifts in
06:29the phenotype,
06:30down regulation of FOXP3 and
06:32up regulation of regulation of
06:32CD226 in circling Tregs as
06:35well.
06:36And, I guess, not shown
06:38here is, we also see
06:40a
06:41relative trend towards decreased suppressive
06:43function in circling Tregs.
06:46In one patient who we
06:48were able to collect both
06:49pre and post treatment,
06:52tumor samples,
06:53we ran single cell RNA
06:54and T cell receptor sequencing.
06:56And what we observed was
06:57that, at the post combination
07:00treatments
07:01sample, we do see an
07:02infiltration of,
07:03the absolute quantity of,
07:06infiltrating T cells as represented
07:08by CD three staining,
07:10but also a shift in
07:11the the amino phenotype. So
07:13we see a much larger
07:14expansion of
07:16effector
07:17CDT cells,
07:19in addition to actual clonal
07:20expansion.
07:22But maybe most interesting to
07:24us based off of our
07:25preclinical observations was that if
07:27we were to take the
07:28t cell receptor sequence and
07:29use it as a molecular
07:30barcode
07:31and track what is the
07:32phenotype of regulatory t cells,
07:35what we observe is that
07:36prior to treatments, regulatory t
07:38cells have a very distinct
07:40suppressive phenotype.
07:42And what's shown here are
07:44all of the regulatory T
07:46cell clonotypes, which are confined
07:47to one phenotypic cluster.
07:50But following treatment, we actually
07:51see increase in the clonal
07:53overlap across different
07:54c four effector populations.
07:57And this is interesting to
07:58us because we would hypothesize
07:59that disabling reg TIGIT signaling
08:02would destabilize regulatory t cell
08:04phenotypes.
08:06And so, this is,
08:08obviously in
08:10preliminary data and data that
08:12we're still working on generating,
08:13but,
08:14it does play in line
08:15with the preclinical,
08:17hypothesis
08:18going in,
08:19in a regulatory t cell
08:25manner.
08:26But what we're also interested
08:28in trying to understand is
08:29whether there are bidirectional interactions
08:31that are occurring. And so
08:33a very talented graduate student
08:34in our group is currently
08:36working on what is the
08:37bidirectional signaling
08:39that is occurring and has
08:41generated some very interesting data
08:42to suggest that regulatory T
08:44cell interactions
08:46with glioblastoma cancer cells actually
08:48causes shift towards more mesenchymal
08:50like aggressive phenotypes
08:53and that this
08:54interaction is regulatory
08:56Treg specific
08:58and can be reversed with
09:00t shirt blockade.
09:02But that environmental context matters.
09:04And so
09:05when thinking about the heterogeneity
09:07within
09:08the solid tumor microenvironments,
09:10we also take into consideration
09:12metabolic and,
09:15other
09:16other conditions such as hypoxia.
09:18And that potentially, this may
09:19lead to avenues for additional
09:22therapeutic targeting.
09:24And so with that, I'd
09:25just like to thank,
09:26the patients and families who
09:28have made this work possible
09:29and all of our, human
09:31work possible
09:32in addition to, doctor David
09:34Haffler, who has been my
09:36mentor during my time here
09:37at Yale.
09:38In addition to,
09:40the folks in our group,
09:41the greater Hafler lab group,
09:42and all of our collaborators
09:43around
09:44the medical school, including,
09:46the support of leadership within
09:48the cancer center.
09:49And,
09:52well represented here is also
09:54leadership within the core facilities
09:56who have also helped us
09:57make, this possible, including Waelin
09:59and Leslie.