DDPH对heccm诱导的肺血管周细胞增殖和免疫表型的影响。

Y Yuan, D Che, M Xiong
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引用次数: 0

摘要

为了研究1-(2,6 -二甲基苯氧基)-2-(3,4 -二甲氧基苯乙胺)丙烷盐酸(DDPH)对猪肺动脉缺氧内皮细胞条件培养基(HECCM)诱导的新生大鼠肺血管周细胞增殖和免疫表型的影响,将培养的周细胞按所使用的内皮细胞条件培养基(ECCM)分为4组:常氧ECCM (NECCM)组、NECCM + DDPH组、HECCM组和HECCM + DDPH组。采用细胞培养、免疫细胞化学染色、图像分析和流式细胞术等方法研究了HECCM和DDPH对周细胞α -平滑肌肌动蛋白(α -sm - actin)抗原、CD34抗原、S-100抗原和增殖细胞核抗原(PCNA)表达及细胞周期的影响。结果表明,hecm组周细胞α - sm - actin抗原阳性表达强于其他3组,而CD34抗原和S-100抗原呈阴性表达。α - sm - actin抗原、CD34抗原和S-100抗原在NECCM、NECCM + DDPH和HECCM + DDPH组中表达阳性;α - sm - actin和PCNA在HECCM组的表达分别是NECCM组的1.32倍(P < 0.01)和1.24倍(P < 0.05),是HECCM + DDPH组的1.30倍(P < 0.01)和1.21倍(P < 0.05)。与NECCM、HECCM + DDPH组相比,HECCM组GO-G1期细胞比例分别降低了11.7%和9.1%,S期细胞比例分别提高了5.6%和4.2%,G2-M期细胞比例分别提高了6.1%和4.9%。DDPH对hecm诱导周细胞α - sm - actin和PCNA合成增加的抑制率分别为23.4%和17.1%。对GO-G1期到S期增加的周细胞的抑制率为8.3%。这些结果表明,DDPH可以直接抑制HECCM诱导的平滑肌样细胞的周细胞增殖和免疫表型转化。
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Effects of DDPH on HECCM-induced proliferation and immunophenotypes of the pulmonary vascular pericytes.

In order to study the effects of 1-(2, 6-dimethylphenoxy)-2-(3, 4-dimethoxyphenylethylamino) propane hydrochloride (DDPH) on proliferation and immunophenotypes of newborn rat pulmonary vascular pericytes induced by hypoxic endothelial cell conditioned medium (HECCM) from porcine pulmonary arteries, the cultured pericytes were divided into 4 groups according to the endothelial cell conditioned medium (ECCM) used: normoxic ECCM (NECCM) group, NECCM + DDPH group, HECCM group and HECCM + DDPH group. Cell culture, immunocytochemical staining, image analysis and flow cytometric method were used to investigate the effects of HECCM and DDPH on the expression of alpha-smooth muscle actin (alpha-SM-Actin) antigen, CD34 antigen, S-100 antigen and proliferating cell nuclear antigen (PCNA) and cell cycle in pericytes. The results showed that the alpha-SM-Actin antigen in the pericytes in HECCM group was stronger positively expressed than in the other three groups, but CD34 antigen and S-100 antigen were negatively expressed. The expression of alpha-SM-Actin antigen, CD34 antigen and S-100 antigen was positive in the groups of NECCM, NECCM + DDPH and HECCM + DDPH; The expression of alpha-SM-Actin and PCNA in HECCM group was 1.32 times (P < 0.01) and 1.24 times (P < 0.05) that in NECCM group, 1.30 times (P < 0.01) and 1.21 times (P < 0.05) that in HECCM + DDPH group, respectively. The percentage of the cells in the GO-G1 phase in the HECCM group was lower by 11.7% and 9.1%, in S phase higher by 5.6% and 4.2%, in G2-M phase higher by 6.1% and 4.9% than in the groups of NECCM, HECCM + DDPH, respectively. The inhibitory rate of DDPH on the increased alpha-SM-Actin and PCNA syntheses in pericytes induced by HECCM were 23.4% and 17.1% respectively. The inhibitory rate on the increased pericytes from GO-G1 phase to S phase was 8.3%. These results suggest that DDPH can directly inhibit pericytes from proliferation and immunophenotypical transformation of smooth muscle-like cells induced by HECCM.

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