PGK1 赖氨酸 323 的乙酰化促进腔 A 型乳腺癌细胞的糖酵解、细胞增殖和转移。
Acetylation of PGK1 at lysine 323 promotes glycolysis, cell proliferation, and metastasis in luminal A breast cancer cells.
机构信息
Research Institute of Medicine and Pharmacy, Qiqihar Medical University, Qiqihar, Heilongjiang, China.
Department of Medical Technology, Qiqihar Medical University, Qiqihar, Heilongjiang, China.
出版信息
BMC Cancer. 2024 Aug 27;24(1):1054. doi: 10.1186/s12885-024-12792-8.
BACKGROUND
In prior research employing iTRAQ (Isobaric Tags for Relative and Absolute Quantitation) technology, we identified a range of proteins in breast cancer tissues exhibiting high levels of acetylation. Despite this advancement, the specific functions and implications of these acetylated proteins in the context of cancer biology have yet to be elucidated. This study aims to systematically investigate the functional roles of these acetylated proteins with the objective of identifying potential therapeutic targets within breast cancer pathophysiology.
METHODS
Acetylated targets were identified through bioinformatics, with their expression and acetylation subsequently confirmed. Proteomic analysis and validation studies identified potential acetyltransferases and deacetylases. We evaluated metabolic functions via assays for catalytic activity, glucose consumption, ATP levels, and lactate production. Cell proliferation and metastasis were assessed through viability, cycle analysis, clonogenic assays, PCNA uptake, wound healing, Transwell assays, and MMP/EMT marker detection.
RESULTS
Acetylated proteins in breast cancer were primarily involved in metabolism, significantly impacting glycolysis and the tricarboxylic acid cycle. Notably, PGK1 showed the highest acetylation at lysine 323 and exhibited increased expression and acetylation across breast cancer tissues, particularly in T47D and MCF-7 cells. Notably, 18 varieties acetyltransferases or deacetylases were identified in T47D cells, among which p300 and Sirtuin3 were validated for their interaction with PGK1. Acetylation at 323 K enhanced PGK1's metabolic role by boosting its activity, glucose uptake, ATP production, and lactate output. This modification also promoted cell proliferation, as evidenced by increased viability, S phase ratio, clonality, and PCNA levels. Furthermore, PGK1-323 K acetylation facilitated metastasis, improving wound healing, cell invasion, and upregulating MMP2, MMP9, N-cadherin, and Vimentin while downregulating E-cadherin.
CONCLUSION
PGK1-323 K acetylation was significantly elevated in T47D and MCF-7 luminal A breast cancer cells and this acetylation could be regulated by p300 and Sirtuin3. PGK1-323 K acetylation promoted cell glycolysis, proliferation, and metastasis, highlighting novel epigenetic targets for breast cancer therapy.
背景
在先前使用 iTRAQ(相对和绝对定量的同重同位素标记)技术的研究中,我们在乳腺癌组织中鉴定出了一系列高水平乙酰化的蛋白质。尽管取得了这一进展,但这些乙酰化蛋白在癌症生物学中的具体功能和意义仍有待阐明。本研究旨在系统研究这些乙酰化蛋白的功能作用,以期确定乳腺癌病理生理学中的潜在治疗靶点。
方法
通过生物信息学鉴定乙酰化靶标,随后验证其表达和乙酰化。蛋白质组分析和验证研究鉴定了潜在的乙酰转移酶和去乙酰化酶。我们通过测定催化活性、葡萄糖消耗、ATP 水平和乳酸生成来评估代谢功能。通过细胞活力、周期分析、集落形成实验、PCNA 摄取、划痕愈合实验、Transwell 实验和 MMP/EMT 标志物检测来评估细胞增殖和转移。
结果
乳腺癌中的乙酰化蛋白主要参与代谢,对糖酵解和三羧酸循环有显著影响。值得注意的是,PGK1 在赖氨酸 323 处的乙酰化程度最高,并且在乳腺癌组织中特别是在 T47D 和 MCF-7 细胞中表达和乙酰化水平均升高。在 T47D 细胞中鉴定出 18 种乙酰转移酶或去乙酰化酶,其中 p300 和 Sirtuin3 被验证与 PGK1 相互作用。PGK1 在 323 K 处的乙酰化修饰增强了其代谢作用,提高了其活性、葡萄糖摄取、ATP 生成和乳酸生成。这种修饰还促进了细胞增殖,表现为细胞活力、S 期比例、集落形成能力和 PCNA 水平增加。此外,PGK1-323 K 乙酰化促进了转移,改善了伤口愈合、细胞侵袭,并上调了 MMP2、MMP9、N-钙黏蛋白和波形蛋白,同时下调了 E-钙黏蛋白。
结论
PGK1-323 K 乙酰化在 T47D 和 MCF-7 腔 A 型乳腺癌细胞中显著升高,并且这种乙酰化可以被 p300 和 Sirtuin3 调节。PGK1-323 K 乙酰化促进了细胞糖酵解、增殖和转移,为乳腺癌治疗提供了新的表观遗传靶点。
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