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Immunohistochemical analysis of MCT1, MCT2 and MCT4 expression in rat plantaris muscle

机译:大鼠足底肌中MCT1,MCT2和MCT4表达的免疫组织化学分析

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摘要

We addressed the need for histological assessment of myocellular domains occupied by monocarboxylate transporters (MCT1, MCT2 and MCT4). From the perspective of lactate shuttle hypotheses we posited that MCT1 would be highly expressed in oxidative fibres, whereas MCT4 would be found in highly glycolytic fibres. Furthermore, we hypothesized that MCT1 would be detected at interfibrillar as well as at subsarcolemmal and sarcolemmal cell domains, whereas MCT2 and MCT4 abundances would be most prominent at the sarcolemma. To test these hypotheses, we examined cellular locations of MCT1, MCT2 and MCT4 transporter proteins in different fibre types (slow oxidative, SO; fast oxidative glycolytic, FOG; fast glycolytic, FG) in rat plantaris muscles by the avidin–biotin complex (ABC) as well as other methods. The plantaris was used as it is a mixed fibre skeletal muscle. MCTs, glucose transporter (GLUT4) protein, and mitochondrial constituent cytochrome oxidase (COX) abundances were assessed by immunohistochemistry and Western blotting using affinity-purified antibodies. The staining method was specific and stable, which allowed for semiquantitative assessment of MCT expression. As well, confocal laser scanning microscopy assessed MCT isoform localizations. Findings of the present study were: (1) MCT1 is located at the sarcolemma and throughout the cell interior in SO and FOG fibres where the mitochondrial reticulum was present; (2) in contrast, MCT4 was highly expressed in the sarcolemmal domain of FG and FOG fibres but poorly expressed in SO fibres; and (3) confocal laser-scanning microscopy demonstrated that MCT1 and COX are co-localised at both interfibrillar and subsarcolemmal cell domains, whereas MCT2 is only faintly detected at the sarcolemma of oxidative fibres. MCTs and associated proteins are positioned to facilitate the function of the lactate shuttles.
机译:我们满足了对由单羧酸盐转运蛋白(MCT1,MCT2和MCT4)占据的肌细胞结构域进行组织学评估的需求。从乳酸穿梭假说的观点出发,我们假设MCT1在氧化纤维中高表达,而MCT4在高糖酵解纤维中发现。此外,我们假设MCT1将在纤维间以及在肌膜下和肌膜下的细胞域中检测到,而MCT2和MCT4的丰度在肌膜中最突出。为了检验这些假设,我们通过抗生物素蛋白-生物素复合物(ABC)检查了大鼠plant肌中不同纤维类型(慢氧化,SO;快速氧化糖酵解,FOG;快速糖酵解,FG)中MCT1,MCT2和MCT4转运蛋白的细胞位置)以及其他方法。使用plant骨是因为它是混合纤维骨骼肌。 MCT,葡萄糖转运蛋白(GLUT4)蛋白和线粒体组成细胞色素氧化酶(COX)的丰度通过亲和纯化的抗体通过免疫组织化学和Western印迹进行了评估。染色方法特异且稳定,可用于MCT表达的半定量评估。同样,共聚焦激光扫描显微镜评估了MCT亚型的定位。本研究的发现是:(1)MCT1位于线粒体网孔处的SO和FOG纤维的肌膜处和整个细胞内部。 (2)相反,MCT4在FG和FOG纤维的肌膜区高表达,而在SO纤维中表达低; (3)共聚焦激光扫描显微镜证明,MCT1和COX共同定位在原纤维间和肌膜下细胞域,而MCT2仅在氧化纤维的肌膜处微弱地检测到。 MCT和相关蛋白的位置有助于乳酸梭的功能。

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