MMP2 and TLRs modulate immune responses in the tumor microenvironment
Luciana R. Muniz-Bongers, Christopher B. McClain, Mansi Saxena, Gerold Bongers, Miriam Merad, Nina Bhardwaj
Luciana R. Muniz-Bongers, Christopher B. McClain, Mansi Saxena, Gerold Bongers, Miriam Merad, Nina Bhardwaj
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Research Article Immunology Oncology

MMP2 and TLRs modulate immune responses in the tumor microenvironment

Abstract

The presence of an immunosuppressive tumor microenvironment is a major obstacle in the success of cancer immunotherapies. Because extracellular matrix components can shape the microenvironment, we investigated the role of matrix metalloproteinase 2 (MMP2) in melanoma tumorigenesis. We found that MMP2 signals proinflammatory pathways on antigen presenting cells, and this requires both TLR2 and TLR4. B16 melanoma cells that express MMP2 at baseline have slower kinetics in Tlr2–/– Tlr4–/– mice, implicating MMP2 in promoting tumor growth. Indeed, Mmp2 overexpression in B16 cells potentiated rapid tumor growth, which was accompanied by reduced intratumoral cytolytic cells and increased M2 macrophages. In contrast, knockdown of Mmp2 slowed tumor growth and enhanced T cell proliferation and NK cell recruitment. Finally, we found that these effects of MMP2 are mediated through dysfunctional DC–T cell cross-talk as they are lost in Batf3–/– and Rag2–/– mice. These findings provide insights into the detrimental role of endogenous alarmins like MMP2 in modulating immune responses in the tumor microenvironment.

Authors

Luciana R. Muniz-Bongers, Christopher B. McClain, Mansi Saxena, Gerold Bongers, Miriam Merad, Nina Bhardwaj

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Figure 2

MMP2 binds and precipitates with TLR2 and TLR4.

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MMP2 binds and precipitates with TLR2 and TLR4. (A and B) HEK293T cotran...
(A and B) HEK293T cotransfection followed by Flag pull-down using magnetic beads. Mmp2-Flag was cotransfected with Tlr2-HA, Tlr4-Myc, or both plasmids (A). Mmp9-Flag cotransfection with Tlr-plasmids or Myd88-HA plasmid was also evaluated (B). (C) Reverse co-IP of Mmp2-Flag or Mmp9-Flag cotransfected with Tlr2-HA, Tlr4-Myc, or both plasmids. HA or Myc pull-down using anti-HA agarose or Anti–c-MYC agarose beads. (D) Schematic of the different MMP2 constructs used in the co-IP to identify the binding domain. (E and F) Different MMP2 domains were deleted or expressed alone and tested for co-IP with Tlr2-HA. Black line indicates where membrane ends/was cut. All transfections were performed using Lipofectamine 3000, and protein was extracted 20–24 hours after transfection. IP, immunoprecipitation; IB, immunoblotting; WCE, whole-cell extract; Δ, deletion.