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Expression of smooth muscle caldesmon in developing chicken gizzard.

机译:发育中的鸡g中平滑肌caldesmon的表达。

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Caldesmon is an actin/calmodulin/tropomyosin protein located in the thin filaments of smooth muscle cells and microfilaments of nonmuscle cells. Two isoforms of caldesmon, h- and l-types, shown to exist in vertebrate smooth and nonmuscle cells respectively, are produced by alternative splicing of the caldesmon mRNA encoded by a single gene. To study the expression of smooth muscle specific h-caldesmon during the differentiation of mesenchymal cells into smooth muscle cells, soluble protein and total RNA from the gizzard primordium in the gut region of 5-day and gizzards of 7-, 9-, 13-, 17- and 21-day embryos and 2-days post-hatch chicks were extracted and analyzed for caldesmon expression at both protein and mRNA levels. Western blot analysis of proteins and immunofluorescence microscopy of tissue section were carried out using an antibody specific for h-caldesmon. Total RNA was analyzed by Northern blotting using a caldesmon cDNA probe, and h- and l-caldesmon cDNAs were identified due to the difference in their molecular sizes (4.8 and 4.1 kb respectively). The mRNA was also analyzed by reverse transcribed-polymerase chain reaction (RT-PCR) and Southern blot analysis. Our results show that the I-caldesmon mRNA was expressed at higher levels in the gizzard primordium during the early stages of development, and decreased gradually during growth. The h-caldesmon protein and mRNA, not expressed at day 5, is minimally expressed at day 7 and is fully turned on by day 9. Additionally, sequence analyses of the RT-PCR products of I-caldesmon showed that it lacked the spacer region, as predicted. RT-PCR analysis of total RNA gave two h-caldesmon fragments. These two fragments were identified as two different isoforms of h-caldesmon since they both contained the spacer region. They also showed homology in the region of exon 4 had differences in the region of exon 3b.
机译:Caldesmon是一种肌动蛋白/钙调蛋白/原肌球蛋白,位于平滑肌细胞的细丝和非肌细胞的微丝中。通过单独剪接由单个基因编码的caldesmon mRNA,产生了分别在脊椎动物的平滑肌和非肌肉细胞中分别存在的caldesmon的两种同工型,h型和l型。研究间充质细胞向平滑肌细胞分化过程中平滑肌特异性h-caldesmon的表达,肠胃区域5天的izz原基和7-,9-,13- g的可溶性蛋白和总RNA提取17、21和21天的胚胎以及孵化后2天的雏鸡,并在蛋白质和mRNA水平上分析卡尔德斯蒙表达。蛋白质的蛋白质印迹分析和组织切片的免疫荧光显微镜检查是使用对h-caldesmon特异的抗体进行的。使用caldesmon cDNA探针通过Northern印迹分析总RNA,并且由于分子大小的差异(分别为4.8和4.1 kb)而鉴定出h-和l-caldesmon cDNA。还通过逆转录聚合酶链反应(RT-PCR)和Southern印迹分析对mRNA进行了分析。我们的结果表明,I-caldesmon mRNA在发育初期在g原基中表达较高,而在生长过程中逐渐降低。在第5天未表达的h-caldesmon蛋白和mRNA在第7天表达最少,并在第9天完全开启。此外,对I-caldesmon RT-PCR产物的序列分析表明,其缺少间隔区,正如预期的那样。总RNA的RT-PCR分析给出了两个h-caldesmon片段。由于这两个片段均包含间隔区,因此将其鉴定为h-caldesmon的两种不同同工型。他们还显示外显子4区域的同源性在外显子3b区域具有差异。

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