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Technical note: Protocol for electrophoretic separation of bovine myosin heavy chain isoforms and comparison to immunohistochemistry analysis

机译:技术说明:牛肌苷重链同种型的电泳分离协议,与免疫组织化学分析的比较

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摘要

Myosin heavy chain (MyHC) isoform composition is a primary determinant of contractile speed of muscle fibers. Currently, bovine MyHC isoforms are evaluated using time-consuming histochemical analysis by immunflourescence or ATPase activity. Electrophoretic separation of MyHC isoforms is more rapid; however, a reliable procedure without use of gradients has not been validated for cattle. Therefore, our objectives were to develop and validate a procedure for separating bovine MyHC isoforms (I, IIa, and IIx) using sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE), and compare results to immunohistochemistry (IHC) analysis. Muscle samples were collected from masseter, sternomandibularis, diaphragm, longissimus lumborum, and cutaneous trunci within 1.5 h postmortem. To determine appropriate conditions for electrophoretic separation, several parameters of gel composition were varied. Bovine MyHC isoforms were clearly separated by increasing glycerol content of polyacrylamide gels to 37%. Identity of MyHC isoforms was confirmed using western blotting. Percent MyHC composition evaluated by gel electrophoresis was consistent with IHC (P 0.2). Thus, SDS-PAGE produces clear separation of MyHC isoforms, and is a viable alternative to IHC-based methods.
机译:肌球蛋白重链(MYHC)同种型组合物是肌纤维的收缩速度的主要决定因素。目前,使用免疫荧光或ATPase活性使用耗时的组织化学分析来评估牛MyHC同种型。 MyHC同种型的电泳分离更快;然而,不使用梯度的可靠程序尚未为牛验证。因此,我们的目标是通过使用十二烷基硫酸钠聚丙烯酰胺凝胶电泳(SDS-PAGE)来开发和验证分离牛MyHC同种型(I,IIA和IIX)的程序,并将结果与​​免疫组织化学(IHC)分析进行比较。从Masseter,胸骨,胸腔,膈肌,Longissimus Lumborum和1.5小时后的皮肤trunci收集肌肉样品。为了确定电泳分离的适当条件,改变了几种凝胶组合物的参数。牛MyHC的同种型进行了明确通过增加聚丙烯酰胺凝胶的甘油含量37%分离。使用Western Blotting确认了MyHC同种型的身份。通过凝胶电泳评估的MyHC组成百分比与IHC(P> 0.2)一致。因此,SDS-PAGE会产生明确的MYHC同种型分离,并且是基于IHC的方法的可行替代方案。

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