Literature DB >> 30395269

Acetylation of ACAP4 regulates CCL18-elicited breast cancer cell migration and invasion.

Xiaoyu Song1,2, Wei Liu1,2, Xiao Yuan1,3, Jiying Jiang1,2, Wanjuan Wang4, McKay Mullen2, Xuannv Zhao1, Yin Zhang1,4, Fusheng Liu1,4, Shihao Du1,4, Adeel Rehman1, Ruijun Tian3, Jian Li2, Andra Frost5, Zhenwei Song1, Hadiyah-Nicole Green2, Calmour Henry2, Xing Liu1,2, Xia Ding4,2, Dongmei Wang1, Xuebiao Yao1.   

Abstract

Tumor metastasis represents the main causes of cancer-related death. Our recent study showed that chemokine CCL18 secreted from tumor-associated macrophages regulates breast tumor metastasis, but the underlying mechanisms remain less clear. Here, we show that ARF6 GTPase-activating protein ACAP4 regulates CCL18-elicited breast cancer cell migration via the acetyltransferase PCAF-mediated acetylation. CCL18 stimulation elicited breast cancer cell migration and invasion via PCAF-dependent acetylation. ACAP4 physically interacts with PCAF and is a cognate substrate of PCAF during CCL18 stimulation. The acetylation site of ACAP4 by PCAF was mapped to Lys311 by mass spectrometric analyses. Importantly, dynamic acetylation of ACAP4 is essential for CCL18-induced breast cancer cell migration and invasion, as overexpression of the persistent acetylation-mimicking or non-acetylatable ACAP4 mutant blocked CCL18-elicited cell migration and invasion. Mechanistically, the acetylation of ACAP4 at Lys311 reduced the lipid-binding activity of ACAP4 to ensure a robust and dynamic cycling of ARF6-ACAP4 complex with plasma membrane in response to CCL18 stimulation. Thus, these results present a previously undefined mechanism by which CCL18-elicited acetylation of the PH domain controls dynamic interaction between ACAP4 and plasma membrane during breast cancer cell migration and invasion.

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Year:  2018        PMID: 30395269      PMCID: PMC6692856          DOI: 10.1093/jmcb/mjy058

Source DB:  PubMed          Journal:  J Mol Cell Biol        ISSN: 1759-4685            Impact factor:   6.216


  14 in total

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