Hydroxysafflor Yellow A promotes angiogenesis of brain microvascular endothelial cells from ischemia/reperfusion injury via glycolysis pathway in vitro.

Juxuan Ruan, Lei Wang, Ning Wang, Ping Huang, Dennis Chang, Xian Zhou, Saiwang Seto, Dan Li, Jincai Hou
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Abstract

Background: Angiogenesis of brain microvascular endothelial cells (BMECs) after cerebral ischemia was conducive to improving the blood supply of ischemia tissues, which was upregulated by glycolysis. Hydroxysafflor Yellow A (HSYA) mends damaged tissues through increasing angiogenesis.

Methods: HSYA treated proliferation, migration and angiogenesis of BMECs in vitro in vitro during OGD/R. HSYA regulated the key enzymes of glycolysis, such as hexokinase 2 (HK2) and 6-phosphofructo-2-kinase/fructose-2,6-biphosphatase 3 (PFKFB3), glucose uptake and products (pyruvate, ATP and lactate) were detected by western blot and kits, respectively. Scratch wound assay, transwell, tube formation and spheroid sprouting were used to explore the pathway that HSYA recovered migration and angiogenesis of BMECs. We evaluated the potential target of HSYA promoting glycolysis via molecular docking, drug affinity responsive target stability (DARTS) and cellular thermal shift assay (CETSA).

Results: HSYA promoted the proliferation, migration, tube formation and spheroid sprouting of BMECs during OGD/R, and stimulated the expression of tip phenotype marker protein (CD34), and the receptor (Notch-1) that regulated the differentiation of endothelial cells into tip/stalk phenotype. In glycolysis, PFKFB3 expression was upregulated by HSYA; HSYA also improved ATP and pyruvate levels, as well as lactate release after OGD/R. Finally, upregulating VEGFA and p-VEGFR2 of HSYA was weakened because of suppressing glycolysis; the HSYA's improvement of BMECs migration and angiogenesis was attenuated under the inhibition of glycolysis, which confirmed that HSYA were upregulating angiogenesis and expression of VEGFA/VEGFR2 by glycolysis pathway. The result about molecular docking, DARTS and CETSA suggested that PFKFB3 was the possible target of HSYA.

Conclusion: HSYA promotes angiogenesis of BMECs in vitro through the glycolysis mediated VEGFA/VEGFR2 pathway, and PFKFB3 is the potential target of HSYA to heighten glycolysis.

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羟基红花黄色素 A 在体外通过糖酵解途径促进缺血再灌注损伤的脑微血管内皮细胞的血管生成。
背景:脑缺血后脑微血管内皮细胞(BMECs)的血管生成有利于改善缺血组织的血液供应,而糖酵解会上调血管生成。方法:Hydroxysafflor Yellow A(HSYA)通过增加血管生成来修复受损组织。HSYA调节糖酵解的关键酶,如己糖激酶2(HK2)和6-磷酸果糖-2-激酶/果糖-2,6-二磷酸酶3(PFKFB3),葡萄糖摄取和产物(丙酮酸、ATP和乳酸)分别通过Western印迹和试剂盒检测。采用划痕法、Transwell法、管形成法和球形萌发法探讨了HSYA恢复BMECs迁移和血管生成的途径。我们通过分子对接、药物亲和力反应靶点稳定性(DARTS)和细胞热转移试验(CETSA)评估了HSYA促进糖酵解的潜在靶点:结果:HSYA在OGD/R过程中促进了BMECs的增殖、迁移、管形成和球形萌发,并刺激了尖端表型标志蛋白(CD34)和受体(Notch-1)的表达,从而调控内皮细胞向尖端/茎表型分化。在糖酵解方面,HSYA 上调了 PFKFB3 的表达;HSYA 还改善了 ATP 和丙酮酸的水平,以及 OGD/R 后乳酸的释放。最后,HSYA对VEGFA和p-VEGFR2的上调作用因抑制糖酵解而减弱;在抑制糖酵解的条件下,HSYA对BMECs迁移和血管生成的改善作用减弱,证实HSYA通过糖酵解途径上调血管生成和VEGFA/VEGFR2的表达。分子对接、DARTS和CETSA结果表明,PFKFB3可能是HSYA的靶点:结论:HSYA 通过糖酵解介导的 VEGFA/VEGFR2 通路促进体外 BMECs 的血管生成,而 PFKFB3 是 HSYA 促进糖酵解的潜在靶点。
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来源期刊
CiteScore
5.00
自引率
4.00%
发文量
583
审稿时长
62 days
期刊介绍: The Journal of Stroke & Cerebrovascular Diseases publishes original papers on basic and clinical science related to the fields of stroke and cerebrovascular diseases. The Journal also features review articles, controversies, methods and technical notes, selected case reports and other original articles of special nature. Its editorial mission is to focus on prevention and repair of cerebrovascular disease. Clinical papers emphasize medical and surgical aspects of stroke, clinical trials and design, epidemiology, stroke care delivery systems and outcomes, imaging sciences and rehabilitation of stroke. The Journal will be of special interest to specialists involved in caring for patients with cerebrovascular disease, including neurologists, neurosurgeons and cardiologists.
期刊最新文献
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