Trastuzumab/pertuzumab combination therapy stimulates antitumor responses through complement-dependent cytotoxicity and phagocytosis
Li-Chung Tsao, Erika J. Crosby, Timothy N. Trotter, Junping Wei, Tao Wang, Xiao Yang, Amanda N. Summers, Gangjun Lei, Christopher A. Rabiola, Lewis A. Chodosh, William J. Muller, Herbert Kim Lyerly, Zachary C. Hartman
Li-Chung Tsao, Erika J. Crosby, Timothy N. Trotter, Junping Wei, Tao Wang, Xiao Yang, Amanda N. Summers, Gangjun Lei, Christopher A. Rabiola, Lewis A. Chodosh, William J. Muller, Herbert Kim Lyerly, Zachary C. Hartman
View: Text | PDF
Research Article Oncology Therapeutics

Trastuzumab/pertuzumab combination therapy stimulates antitumor responses through complement-dependent cytotoxicity and phagocytosis

Abstract

Two HER2-specific mAbs, trastuzumab and pertuzumab (T+P), combined with chemotherapy comprise standard-of-care treatment for advanced HER2+ breast cancers (BC). While this antibody combination is highly effective, its synergistic mechanism-of-action (MOA) remains incompletely understood. Past studies have suggested that the synergy underlying this combination occurs through the different mechanisms elicited by these antibodies, with pertuzumab suppressing HER2 heterodimerization and trastuzumab inducing antitumor immunity. However, in vivo evidence for this synergy is lacking. In this study, we found that the therapeutic efficacy elicited by their combination occurs through their joint ability to activate the classical complement pathway, resulting in both complement-dependent cytotoxicity and complement-dependent cellular phagocytosis of HER2+ tumors. We also demonstrate that tumor C1q expression is positively associated with survival outcome in HER2+ BC patients and that complement regulators CD55 and CD59 were inversely correlated with outcome, suggesting the clinical importance of complement activity. Accordingly, inhibition of C1q in mice abolished the synergistic therapeutic activity of T+P therapy, whereas knockdown of CD55 and CD59 expression enhanced T+P efficacy. In summary, our study identifies classical complement activation as a significant antitumor MOA for T+P therapy that may be functionally enhanced to potentially augment clinical therapeutic efficacy.

Authors

Li-Chung Tsao, Erika J. Crosby, Timothy N. Trotter, Junping Wei, Tao Wang, Xiao Yang, Amanda N. Summers, Gangjun Lei, Christopher A. Rabiola, Lewis A. Chodosh, William J. Muller, Herbert Kim Lyerly, Zachary C. Hartman

×

Figure 2

Role of FCGR engagements in HER2 mAb antitumor activity.

Options: View larger image (or click on image) Download as PowerPoint
Role of FCGR engagements in HER2 mAb antitumor activity. (A and B) Mouse...
(A and B) Mouse FCGR signaling activation assay. KPL-4 cells were plated and treated with indicated HER2 mAbs concentrations for 1 hour. Jurkat cells containing NFAT-luciferase reporter and expressing mouse FCGR1 (A) and FCGR4 (B) were added to the KPL-4 cells containing antibodies and cocultured for 4 hours. FCGR signaling activation were assessed by luciferase activity quantification. (C and D) Human FCGR signaling activation was similarly quantified with Jurkat-NFAT-Luciferase reporter cells expressing human FCGR1 (C) and FCGR3A (D). (EG) Mouse FCGR signaling activation assays were repeated using murinized HER2 mAbs with the IgG2A isotype. In addition to mFCGR1 (E) and mFCGR4 (F), mouse FCGR3 (G) was tested here since mFCGR3 can be activated by murine antibodies but not human antibodies. All data represents mean ± SEM; n = 4. (HJ) Antigen-binding-fragment F(ab’)2 of the HER2 mAbs were generated and their therapeutic efficacy against HER2+ BC in vivo were compared with the parental antibody, respectively. As described before, KPL-4 cells (5 × 105 cells) were implanted in mammary fat pads of SCID-beige mice and treated with the indicated HER2 mAbs or F(ab’)2 (100 μg per week). (H) Comparison between Trastuzumab versus Trastuzumab-F(ab’)2. (I) Comparison between Pertuzumab versus Pertuzumab-F(ab’)2. (J) Comparison between T+P versus Trastuzumab + Pertuzumab-F(ab’)2 versus Trastuzumab-F(ab’)2 + Pertuzumab. Numbers of mice showing total tumor regression are displayed on the right of the graph. (HJ) n = 8–10 for all groups. Two-way ANOVA with Tukey’s multiple-comparison post hoc test. All data represent mean ± SEM; *P < 0.05, ***P < 0.001, ****P < 0.0001.