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长期培养的成年哺乳动物心肌细胞的DNA合成

DNA synthesis of adult mammalian cardiac muscle cells in long-term culture.

作者信息

Nag A C, Cheng M

出版信息

Tissue Cell. 1986;18(4):491-7. doi: 10.1016/0040-8166(86)90015-7.

DOI:10.1016/0040-8166(86)90015-7
PMID:3750314
Abstract

Adult rat cardiac ventricular muscle cells were isolated and cultured in monolayer for 30-45 days. Most of the cardiac muscle cells undergo external and internal structural alterations, resembling embryonic/neonatal cardiac muscle cells in culture (Nag and Cheng, 1981; Nag et al., 1983). These cultured cells underwent DNA synthesis and mitosis as revealed by autoradiography studies that involved the exposure of the cells to [3H]-thymidine for 24 hr prior to the termination of the culture at selected intervals. During the first week of culture, cardiac muscle cells showed less than 5% labeled cells. The labeling index of myocytes attained a peak in the second week of culture, exhibiting approximately 23% labeled cells. The labeling indices of cardiac muscle cells declined over the period of 30 days of culture. During the end of the incubation period, approximately 4% of the myocytes were labeled. When the extent of the total cell population involved in DNA synthesis was examined by exposing the cells to [3H]-thymidine continuously for long periods of time, it was observed that approximately 26% of the cardiac muscle cells regained the capacity for DNA synthesis during 1-10 days of culture. From day 1 to day 14, approximately 29% of the total muscle cell population was labeled. When the cells were exposed to the radioactive isotope continuously for 30 days, approximately 31% of the cells incorporated radioactive isotope, showing their capacity for DNA synthesis. Approximately 90% of the cardiac muscle cells in long-term culture contained more than one nucleus. The nuclei were often observed in multiples of two. Labeled mitotic apparatus was observed in cardiac myocytes, indicating the replication of DNA, followed by karyokinesis.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

成年大鼠心室肌细胞被分离出来并进行单层培养30至45天。大多数心肌细胞经历了外部和内部结构的改变,类似于培养中的胚胎/新生心肌细胞(纳格和程,1981年;纳格等人,1983年)。如放射自显影研究所显示的,这些培养的细胞经历了DNA合成和有丝分裂,该研究包括在选定的培养间隔结束前24小时,让细胞接触[3H] - 胸腺嘧啶核苷。在培养的第一周,心肌细胞中标记细胞少于5%。心肌细胞的标记指数在培养的第二周达到峰值,约有23%的标记细胞。在30天的培养期内,心肌细胞的标记指数下降。在培养期末,约4%的心肌细胞被标记。当通过长时间持续让细胞接触[3H] - 胸腺嘧啶核苷来检查参与DNA合成的总细胞群体的范围时,观察到约26%的心肌细胞在培养的1至10天内恢复了DNA合成能力。从第1天到第14天,约29%的总肌肉细胞群体被标记。当细胞连续30天接触放射性同位素时,约31%的细胞掺入了放射性同位素,表明它们具有DNA合成能力。长期培养中约90%的心肌细胞含有不止一个细胞核。细胞核常常以两个为倍数出现。在心肌细胞中观察到标记的有丝分裂器,表明DNA复制,随后是核分裂。(摘要截断于250字)

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DNA synthesis of adult mammalian cardiac muscle cells in long-term culture.长期培养的成年哺乳动物心肌细胞的DNA合成
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