首页> 外文期刊>Endocrine journal >Up-Regulation of JAM-1 in AR42J Cells Treated with Activin A and Betacellulin and the Diabetic Regenerating Islets
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Up-Regulation of JAM-1 in AR42J Cells Treated with Activin A and Betacellulin and the Diabetic Regenerating Islets

机译:激活素A和Betacellulin和糖尿病再生岛对AR42J细胞JAM-1的上调

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Pancreatic AR42J cells demonstrate the pluripotency in precursor cells of the gut endoderm and also provide an excellent model system to study the differentiation of the pancreas. Using the mRNA differential display technique, we identified junctional adhesion molecule-1 (JAM-1), a component of the tight junction, was highly up-regulated during the differentiation of AR42J cells, although junctions were not formed. The expression level of JAM-1 showed an up-regulation in the mRNA level after 3 hours and in the protein level after 24 hours in [activin A + betacellulin]-treated AR42J cells. The expressions of its signaling molecules, PAR-3 and atypical PKCλ, also increased after the addition of activin A + betacellulin. When JAM-1 was over-expressed in [activin A + betacellulin]-treated AR42J cells, tagged-JAM-1 was observed in cytoplasm as vesicular structures and JAM-1 was colocalized with Rab3B and Rabl3, members of the Rab family expressed at tight junctions. In streptozotocin-induced regenerating islets, the expression of JAM-1 was also up-regulated in the mRNA level and the protein level. JAM-1 might therefore play an important role in the differentiation of AR42J cells and the regeneration of pancreatic islets.
机译:胰腺AR42J细胞在肠道内胚层的前体细胞中表现出多能性,也为研究胰腺的分化提供了出色的模型系统。使用mRNA差异显示技术,我们确定了AR42J细胞分化过程中紧密连接的一个组成部分-连接粘附分子1(JAM-1)被高度上调,尽管没有形成连接。在[激活素A +β纤维素]处理的AR42J细胞中,JAM-1的表达水平在3小时后mRNA水平上调,在24小时后蛋白水平上调。加入激活素A +β纤维素后,其信号分子PAR-3和非典型PKCλ的表达也增加。当在[激活素A +β纤维素]处理的AR42J细胞中过表达JAM-1时,在细胞质中观察到标记的JAM-1为囊泡结构,并且JAM-1与Rab3B和Rabl3共定位,Rab家族成员在紧密连接。在链脲佐菌素诱导的再生胰岛中,JAM-1的表达在mRNA水平和蛋白质水平上也上调。因此,JAM-1可能在AR42J细胞的分化和胰岛的再生中起重要作用。

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