[Effects of Down-Regulation of PAK1 on Differentiation and Apoptosis of MPN Cells with MPLW515L Gene Mutation and Survival of 6133/MPL Mice].

Qi-Gang Zhang, Shu-Jin Wang, Xiang-Ru Yu, Li-Wei Zhang, Kai-Lin Xu, Chun-Ling Fu
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引用次数: 0

Abstract

Objective: To investigate the effects of down-regulation of p21 activated kinase 1 (PAK1) on the proliferation, differentiation, and apoptosis of myeloproliferative neoplasm (MPN) cells (6133/MPL) with thrombopoietin receptor MPL mutation at codon 515 (MPLW515L) and survival of 6133/MPL mice.

Methods: Interference with the protein level of PAK1 in 6133/MPL cells was assessed using lentivirus-mediated shRNA transfection technology. CCK-8 assay was used to detect the effect of down-regulation of PAK1 on the proliferation viability of 6133/MPL cells, and colony-forming ability was measured by cell counting. Flow cytometry was used to detect the PAK1 kinase activity on the ability of polyploid DNA formation and cell apoptosis in 6133/MPL cells. The expression of cyclin D1, cyclin D3 and apoptosis-related protein Bax was detected by Western blot. The infiltration of tumor cells in spleen and bone marrow of 6133/MPL mice were detected by HE staining.

Results: Down-regulation of PAK1 inhibited the proliferation and reduced the ability of cell colony formation of 6133/MPL cells. After knocking down PAK1, the content of polyploid DNA in 6133/MPL cells increased from 31.8 to 57.5% and 48.0%, and the proportion of apoptosis increased approximately to 10.8%. Down-regulation of PAK1 led to a reduction of infiltration of tumor cells in liver and bone marrow of 6133/MPL mice, thereby prolonging survival time.

Conclusion: Down-regulation of PAK1 can significantly inhibit the growth of 6133/MPL cells, promote the formation of polyploid DNA, induce 6133/MPL cell apoptosis, and prolong the survival time of 6133/MPL mice.

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[下调 PAK1 对 MPLW515L 基因突变的 MPN 细胞分化和凋亡以及 6133/MPL 小鼠存活的影响]
目的研究下调p21活化激酶1(PAK1)对血小板生成素受体MPL密码子515突变(MPLW515L)的骨髓增殖性肿瘤(MPN)细胞(6133/MPL)的增殖、分化和凋亡以及6133/MPL小鼠存活的影响:方法:使用慢病毒介导的 shRNA 转染技术评估了对 6133/MPL 细胞中 PAK1 蛋白水平的干扰。CCK-8检测法检测下调PAK1对6133/MPL细胞增殖活力的影响,细胞计数法测量集落形成能力。流式细胞术检测了 PAK1 激酶活性对 6133/MPL 细胞多倍体 DNA 形成和细胞凋亡能力的影响。通过 Western 印迹检测细胞周期蛋白 D1、细胞周期蛋白 D3 和细胞凋亡相关蛋白 Bax 的表达。HE 染色法检测 6133/MPL 小鼠脾脏和骨髓中肿瘤细胞的浸润情况:结果:PAK1的下调抑制了6133/MPL细胞的增殖并降低了细胞集落形成的能力。敲除 PAK1 后,6133/MPL 细胞中的多倍体 DNA 含量从 31.8% 增加到 57.5% 和 48.0%,细胞凋亡的比例约增加到 10.8%。下调PAK1可减少肿瘤细胞在6133/MPL小鼠肝脏和骨髓中的浸润,从而延长生存时间:结论:下调 PAK1 能显著抑制 6133/MPL 细胞的生长,促进多倍体 DNA 的形成,诱导 6133/MPL 细胞凋亡,延长 6133/MPL 小鼠的存活时间。
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来源期刊
中国实验血液学杂志
中国实验血液学杂志 Medicine-Medicine (all)
CiteScore
0.40
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7331
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