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Spatial and temporal regulation of a foreign gene by a prestalk-specific promoter in transformed Dictyostelium discoideum.

机译:外源基因在转化的盘基网柄菌中的前柄特异性启动子对时空基因的时空调节。

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摘要

We analyzed a developmentally regulated prestalk-specific gene from Dictyostelium discoideum encoding a cathepsin-like protease. A hybrid gene was constructed by fusing 2.5 kilobases of 5' flanking sequences and part of the coding region of the gene in-frame to the Escherichia coli beta-glucuronidase gene and was transformed into D. discoideum cells. In cells transformed with this vector, the gene fusion showed the same temporal regulation as the endogenous gene during multicellular development and, like endogenous prestalk genes, was highly inducible by cyclic AMP in in vitro cell cultures. Moreover, immunofluorescence studies showed that the fusion protein had the same spatial distribution within the migrating pseudoplasmodium as the endogenous gene. The results indicate that the regions of the D. discoideum prestalk-specific cathepsin gene contain all the necessary information for proper temporal, spatial, and cyclic AMP regulation of a prestalk cell-type gene in D. discoideum transformants and leads the way for experiments to identify the cell-type-specific regulatory elements.
机译:我们分析了来自Disctyostelium discoideum的发育调控的前柄特异性基因,该基因编码组织蛋白酶样蛋白酶。通过将2.5千碱基的5'侧翼序列和该基因的部分编码区框内融合到大肠杆菌β-葡糖醛酸糖苷酶基因中,构建了一个杂种基因,并将其转化为D. discoideum细胞。在用该载体转化的细胞中,基因融合在多细胞发育过程中显示出与内源基因相同的时间调控,并且与内源茎基因一样,在体外细胞培养中可被环AMP高度诱导。此外,免疫荧光研究表明,融合蛋白在迁移的拟疟原虫中具有与内源基因相同的空间分布。结果表明,D。discoideum前茎特异性组织蛋白酶基因的区域包含所有必要信息,以适当地对D. discoideum转化子中的前茎细胞类型基因进行时间,空间和循环AMP调节,从而为实验提供了途径确定特定于细胞类型的调控元件。

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