Safety and antitumor activity of recombinant soluble Apo2 ligand
Avi Ashkenazi, … , Zahra Shahrokh, Ralph H. Schwall
Avi Ashkenazi, … , Zahra Shahrokh, Ralph H. Schwall
Published July 15, 1999
Citation Information: J Clin Invest. 1999;104(2):155-162. https://doi.org/10.1172/JCI6926.
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Article

Safety and antitumor activity of recombinant soluble Apo2 ligand

Abstract

TNF and Fas ligand induce apoptosis in tumor cells; however, their severe toxicity toward normal tissues hampers their application to cancer therapy. Apo2 ligand (Apo2L, or TRAIL) is a related molecule that triggers tumor cell apoptosis. Apo2L mRNA is expressed in many tissues, suggesting that the ligand may be nontoxic to normal cells. To investigate Apo2L’s therapeutic potential, we generated in bacteria a potently active soluble version of the native human protein. Several normal cell types were resistant in vitro to apoptosis induction by Apo2L. Repeated intravenous injections of Apo2L in nonhuman primates did not cause detectable toxicity to tissues and organs examined. Apo2L exerted cytostatic or cytotoxic effects in vitro on 32 of 39 cell lines from colon, lung, breast, kidney, brain, and skin cancer. Treatment of athymic mice with Apo2L shortly after tumor xenograft injection markedly reduced tumor incidence. Apo2L treatment of mice bearing solid tumors induced tumor cell apoptosis, suppressed tumor progression, and improved survival. Apo2L cooperated synergistically with the chemotherapeutic drugs 5-fluorouracil or CPT-11, causing substantial tumor regression or complete tumor ablation. Thus, Apo2L may have potent anticancer activity without significant toxicity toward normal tissues.

Authors

Avi Ashkenazi, Roger C. Pai, Sharon Fong, Susan Leung, David A. Lawrence, Scot A. Marsters, Christine Blackie, Ling Chang, Amy E. McMurtrey, Andrea Hebert, Laura DeForge, Iphigenia L. Koumenis, Derf Lewis, Louise Harris, Jeanine Bussiere, Hartmut Koeppen, Zahra Shahrokh, Ralph H. Schwall

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Figure 1

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Oligomeric state and bioactivity of bacterially produced soluble human A...
Oligomeric state and bioactivity of bacterially produced soluble human Apo2L. (a) Denaturing SDS-PAGE analysis of purified soluble Apo2L (2 μg) without (–) or with (+) reduction by 25 mM of DTT. Molecular weight markers are shown in the left lane. The gel was stained with silver. Identical results were obtained when reduced and nonreduced Apo2L was run on separate gels (not shown). (b) Nondenaturing chromatographic analysis of purified soluble Apo2L. Purified Apo2L (2 μg) was run on a Superose 12 size-exclusion HPLC column in a buffer containing 400 mM ammonium sulfate and 13 mM sodium phosphate (pH 6.5) and was detected by absorbance at 214 nm. The elution time of molecular weight markers is indicated by arrows. The peak appearing at 29–30 minutes is from buffer elution at the included volume of the column. (c) Measurement of Apo2L concentration. Representative standard curve for Apo2L concentration as determined by ELISA with 2 monoclonal anti-human Apo2L antibodies that recognize epitopes in Apo2L’s extracellular region. (d) Measurement of Apo2L bioactivity. Representative standard curve for Apo2L cytotoxicity toward SK-MES-1.