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单只兔胃平滑肌细胞肌球蛋白重链SMB的表达与缩短速度。

Single rabbit stomach smooth muscle cell myosin heavy chain SMB expression and shortening velocity.

作者信息

Eddinger T J, Meer D P

机构信息

Department of Biology, Marquette University, Milwaukee, Wisconsin 5320l-1881, USA.

出版信息

Am J Physiol Cell Physiol. 2001 Feb;280(2):C309-16. doi: 10.1152/ajpcell.2001.280.2.C309.

Abstract

Isolated single smooth muscle cells (SMCs) from different regions of the rabbit stomach were used to determine a possible correlation between unloaded shortening velocity and smooth muscle (SM) myosin heavy chain (MHC) S1 head isoform composition (SMA, no head insert; SMB, with head insert). alpha-Toxin-permeabilized isolated single cells were maximally activated to measure unloaded shortening velocity and subsequently used in an RT-PCR reaction to determine the SMA/SMB content of the same cell. SM MHC SMA and SMB isoforms are uniquely distributed in the stomach with cells from the fundic region expressing little SMB (38.1 +/- 7.3% SMB; n = 16); cells from the antrum express primarily SMB (94.9 +/- 1.0% SMB; n = 16). Mean fundic cell unloaded shortening velocity was 0.014 +/- 0.002 cell lengths/s compared with 0.036 +/- 0.002 for the antrum cells. Unloaded shortening velocity in these cells was significantly correlated with their percent SMB expression (r2 = 0.58). Resting cell length does not correlate with the percent SMB expression (n = 32 cells). Previously published assays of purified or expressed SMA and SMB heavy meromyosin show a twofold difference in actin filament sliding speed in in vitro motility assays. Extrapolation of our data to 0-100% SMB would give a 10-fold range of shortening velocity, which is closer to the approximately 20-fold range reported from various SM tissues. This suggests that mechanisms in addition to the MHC S1 head isoforms regulate shortening velocity.

摘要

采用从兔胃不同区域分离出的单个平滑肌细胞(SMC),以确定无负荷缩短速度与平滑肌(SM)肌球蛋白重链(MHC)S1头部亚型组成(SMA,无头部插入;SMB,有头部插入)之间可能存在的相关性。用α-毒素通透的分离单个细胞被最大程度激活以测量无负荷缩短速度,随后用于逆转录聚合酶链反应(RT-PCR)以确定同一细胞的SMA/SMB含量。SM MHC的SMA和SMB亚型在胃中呈独特分布,胃底区域的细胞几乎不表达SMB(38.1±7.3%SMB;n = 16);胃窦细胞主要表达SMB(94.9±1.0%SMB;n = 16)。胃底细胞的平均无负荷缩短速度为0.014±0.002细胞长度/秒,而胃窦细胞为0.036±0.002。这些细胞的无负荷缩短速度与其SMB表达百分比显著相关(r2 = 0.58)。静息细胞长度与SMB表达百分比无关(n = 32个细胞)。先前发表的关于纯化或表达的SMA和SMB重酶解肌球蛋白的分析表明,在体外运动分析中,肌动蛋白丝滑动速度存在两倍差异。将我们的数据外推至0 - 100%SMB,将得到10倍的缩短速度范围,这更接近各种SM组织报道的约20倍范围。这表明除了MHC S1头部亚型外,还有其他机制调节缩短速度。

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