Thomas Huckaba PhD

Thomas Huckaba PhD

Assistant Professor

While the work in my laboratory has focused on anumber of topics, I am the PI of one of

the three projects on Xavier’s RCMI grant. Thisproject involves the design and testing of

PROTAC molecules to treat non-small cell lungcancer via the degradation of oncogenic forms of

anaplastic lymphoma kinase.

Anaplastic lymphoma kinase(ALK) is a receptor tyrosine kinase that was first

identified in a chromosomaltranslocation associated with anaplastic large cell lymphoma,

a subtype of T-cellnon-Hodgkin’s lymphoma. This chromosomal translocation generates

a truncated form of the ALKprotein containing the tyrosine kinase domain fused to a

dimerization motif,generating a cytoplasmic, constitutively active form of ALK that serves

as a potent oncogenicdriver. Since this initial discovery, similar ALK fusion proteins have

also been found in diffuselarge B-cell lymphoma, inflammatory myofibroblastic tumor,

breast cancer, colorectalcancer, esophageal squamous cell cancer, renal cell cancer, and

non-small-cell lung cancer(NSCLC). ALK inhibitors have been developed for the

treatment of patients withadvanced ALK -rearranged (i.e., ALK-positive) NSCLC, but

mean time to relapse is 11months, due to mutations in the inhibitor binding site of ALK.

Second- and third-generationinhibitors have been approved, but each suffer from

suppressor mutations overtime. Rather than continue to develop mutation-resistant

inhibitors, we are insteadtargeting ALK for degradation via PROTACs.

Proteolysis-targetingchimeras (PROTACs) are small, bifunctional molecules that

contain a warhead domainspecific to the targeted protein of interest coupled by a short

linker to an E3 ubiquitinligase binding domain. These small molecules promote

ubiquitination andsubsequent proteosomal degradation of the target protein. Since their

initial description in 2001,development of PROTACs targeting over 60 separate proteins

have been published. Usingthis technique to degrade pathological proteins has the

added benefit that PROTACscan often be used at concentrations significantly lower than

standard inhibitors, asthere is no need for PROTACs to be present at stoichiometric

concentrations. Once aPROTAC induces ubiquitination of the target protein, the protein

is degraded and the PROTACis free to bind another protein and repeat the cycle. Finally,

because PROTACs do not haveto bind the active site of their target, this proteolytic

alternative tostoichiometric inhibition has greater flexibility in the design of the warhead

targeting motif.

We have designed andsynthesized small molecule PROTACs to efficiently induce

degradation of ALK fusionproteins and have investigated their therapeutic potential in

ALK-positive NSCLC models in vitro and in vivo. Ourpreliminary data strongly suggest

that targeting ALKdegradation is a novel and potentially effective therapeutic approach

for the treatment of NSCLCrelapsed from ALK inhibitors. Importantly, our PROTACs

induce the degradation ofboth “wild type” dimerized ALK, as well as ALK with suppressor

mutations that conferresistance to FDA-approved inhibitors. We are now in the process

of optimizing our PROTACsfor greater potency (they are already effective at single

nanomolar concentrations)and selectivity. Our ongoing work is directed at bringing these

PROTACs intotranslational work to determine therapeutic usefulness.

LCRC Faculty

Yiwei Zhang, PhD
Tulane University School of Medicine