Improving Antibody-Tubulysin Conjugates through Linker Chemistry and Site-Specific Conjugation |
| |
| Authors: | Joseph Z Hamilton Thomas A Pires Jamie A Mitchell Julia H Cochran Kim K Emmerton Margo Zaval Ivan J Stone Martha E Anderson Steven Jin Dr Andrew B Waight Dr Robert P Lyon Dr Peter D Senter Dr Scott C Jeffrey Dr Patrick J Burke |
| |
| Affiliation: | 1. Seagen Inc., 21823 30th Drive SE, Bothell, WA, 98021 USA;2. Department of Chemistry, University of Illinois at Urbana-Champaign, 505 South Mathews Ave., Urbana, IL, 61801 USA;3. Protein Sciences, Discovery Biologics, Merck Research Laboratories, 213 E Grand Ave., South San Francisco, CA, 94080 USA |
| |
| Abstract: | Tubulysins have emerged in recent years as a compelling drug class for delivery to tumor cells via antibodies. The ability of this drug class to exert bystander activity while retaining potency against multidrug-resistant cell lines differentiates them from other microtubule-disrupting agents. Tubulysin M, a synthetic analogue, has proven to be active and well tolerated as an antibody-drug conjugate (ADC) payload, but has the liability of being susceptible to acetate hydrolysis at the C11 position, leading to attenuated potency. In this work, we examine the ability of the drug-linker and conjugation site to preserve acetate stability. Our findings show that, in contrast to a more conventional protease-cleavable dipeptide linker, the β-glucuronidase-cleavable glucuronide linker protects against acetate hydrolysis and improves ADC activity in vivo. In addition, site-specific conjugation can positively impact both acetate stability and in vivo activity. Together, these findings provide the basis for a highly optimized delivery strategy for tubulysin M. |
| |
| Keywords: | Antibodies cancer drug delivery glucuronides tubulysin |
|
|
