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Transcriptional regulation of the KEL gene and Kell protein expression in erythroid and non-erythroid cells

机译:红细胞和非红细胞中KEL基因和Kell蛋白表达的转录调控

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pThe Kell blood-group antigen was originally reported to be a protein expressed in erythroid tissue only. Transcriptional analysis of the iKEL/i promoter activity in human erythroleukaemia K562 and epithelial HeLa cells by electrophoretic mobility-shift and supershift assays, chloramphenicol acetyltransferase assays, co-transfection studies and site-directed mutagenesis provided the following results: (i) the iKEL/i promoter exhibits a strong transcriptional activity in K562 cells and, unexpectedly, a basal non-erythroid activity in HeLa cells, (ii) up-regulation of the 5′ distal promoter activity occurs only in the erythroid context, and (iii) two motifs localized in the exon 1 region, which bind the Sp1/Sp3 and the human GATA-1/Ku70/80 factors, were required for down-regulation of the promoter activity, but inhibition of the promoter activity by the repressing factors in HeLa cells was incomplete. iKEL/i expression in HeLa cells was performed further by primer-extension analysis, which revealed the presence of a low amount of Kell transcript correlating with basal expression of the Kell protein in these cells, as shown by immunopurification and Western-blot analysis. DNA sequencing of the transcript revealed a sequence identical to that obtained from erythroid tissue. In human tissues, iKEL/i expression was investigated by dot-blot analysis and revealed high levels of Kell mRNAs, particularly in brain tissues, testis and lymphoid tissues. Moreover, most tissues analysed exhibited low levels of Kell transcripts. The Kell protein was also detected by immunohistochemistry in the Sertoli cells of the testis and in lymphoid tissues like spleen and tonsil, specifically localized in the follicular dendritic cells. Altogether, the results indicated that iKEL/i expression is not restricted to erythroid tissue./p
机译:>最初报道,凯尔血型抗原是仅在红系组织中表达的蛋白质。通过电泳迁移率转移和超转移测定,氯霉素乙酰转移酶测定,共转染研究和定点诱变对人红白血病K562和上皮HeLa细胞中 KEL 启动子活性的转录分析提供了以下结果:( i) KEL 启动子在K562细胞中表现出很强的转录活性,并且出乎意料地在HeLa细胞中具有基础的非红系活性,(ii)5'末端启动子活性的上调仅在(iii)定位于外显子1区域的两个基序与Sp1 / Sp3和人类GATA-1 / Ku70 / 80因子结合,是下调启动子活性所必需的,但抑制HeLa细胞中受阻因子的启动子活性不完全。通过引物延伸分析进一步在HeLa细胞中进行 KEL 表达,这表明这些细胞中存在少量与Kell蛋白基础表达相关的Kell转录物,如免疫纯化和Western证实印迹分析。转录物的DNA测序显示与从红系组织获得的序列相同。在人体组织中,通过斑点印迹分析了 KEL 的表达,并发现了高水平的Kell mRNA,特别是在脑组织,睾丸和淋巴组织中。此外,大多数分析的组织显示出低水平的凯尔转录本。还通过免疫组织化学在睾丸的支持细胞以及在脾脏和扁桃体的淋巴样组织中特异性检测到了Kell蛋白,所述淋巴组织特别定位在滤泡树突状细胞中。总之,结果表明 KEL 的表达不仅限于类红细胞组织。

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