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单个心肌细胞中肌球蛋白同工酶的分布。一项免疫组织化学研究。

Distribution of myosin isozymes within single cardiac cells. An immunohistochemical study.

作者信息

Samuel J L, Rappaport L, Mercadier J J, Lompre A M, Sartore S, Triban C, Schiaffino S, Schwartz K

出版信息

Circ Res. 1983 Feb;52(2):200-9. doi: 10.1161/01.res.52.2.200.

Abstract

Isozymes of myosin have been localized with respect to individual cardiac myocytes in hearts from 3-week-old, adult controls, and adult hypophysectomized rats, and in cultured cardiac cells. For this purpose, affinity-purified antibodies reacting specifically with the heavy chains of each of the two major myosin isozymes of adult rat heart, V1 and V3, were used. The distribution of the two isomyosins was determined by double immuno-labeling of the same cell, V1 myosins being revealed by rhodamine and V3 myosins by fluorescein. A procedure is described which allows optimum immunological visualization of the myosin filaments of rod-shaped isolated myocytes. It was found that the response of the cardiac cells to the two antimyosins varied depending on the state of the animal. In 3-week-old rats, all cells were stained with the anti-V1, and almost none with the anti-V3 myosin. In the hypophysectomized animals, on the contrary, all cells were stained with the anti-V3 and none with the anti-V1. A mixed pattern of reactivity was observed in adult controls since 50% of the cells reacted with the anti-V1, 10% with the anti-V3, and 40% with both antibodies. In the latter case, the distributions of V1 and V3 reactivities were homogeneous throughout the cell, and absolutely superimposable. The same double reactivity and homogeneous repartition were observed in cultured cells. These findings indicate that myocytes from adult rat myocardium are heterogeneous in terms of their isomyosins content and show for the first time that two isomyosins can coexist and be equally distributed in one cardiac cell. These observations are relevant to the regulation of individual heart cell contractility.

摘要

已针对3周龄成年对照大鼠、成年垂体切除大鼠心脏中的单个心肌细胞以及培养的心脏细胞,对肌球蛋白同工酶进行了定位。为此,使用了与成年大鼠心脏两种主要肌球蛋白同工酶(V1和V3)的重链特异性反应的亲和纯化抗体。通过对同一细胞进行双重免疫标记来确定两种异肌球蛋白的分布,用罗丹明显示V1肌球蛋白,用荧光素显示V3肌球蛋白。本文描述了一种可对杆状分离心肌细胞的肌球蛋白丝进行最佳免疫可视化的方法。结果发现,心脏细胞对两种抗肌球蛋白的反应因动物状态而异。在3周龄大鼠中,所有细胞均被抗V1抗体染色,几乎没有细胞被抗V3肌球蛋白抗体染色。相反,在垂体切除的动物中,所有细胞均被抗V3抗体染色,没有细胞被抗V1抗体染色。在成年对照动物中观察到一种混合反应模式,因为50%的细胞与抗V1抗体反应,10%的细胞与抗V3抗体反应,40%的细胞与两种抗体都反应。在后一种情况下,V1和V3反应性在整个细胞中的分布是均匀的,并且完全重叠。在培养细胞中也观察到了相同的双重反应性和均匀分布。这些发现表明,成年大鼠心肌中的心肌细胞在其异肌球蛋白含量方面是异质的,并且首次表明两种异肌球蛋白可以共存并在一个心肌细胞中均匀分布。这些观察结果与单个心脏细胞收缩力的调节有关。

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