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Functional domains of the penicillinase repressor of Bacillus licheniformis.

机译:地衣芽孢杆菌青霉素酶阻遏物的功能域。

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摘要

The penicillinase repressor (PENI) negatively regulates expression of the penicillinase gene (penP) in Bacillus licheniformis by binding to its operators located within the promoter region of penP.penI codes for a protein with 128 amino acids. Filter-binding analyses suggest that the active form of the repressor is a dimer. Genetic analyses of PENI derivatives showed that the repressor carrying either a 6-amino-acid deletion near the N terminus or a 14-amino-acid deletion at the C terminus was functionally inactive in vivo. A repressor derivative carrying a 6-amino-acid deletion within its N-terminal region was extensively purified and used in DNA footprinting and subunit cross-linking analyses. The results of these studies showed that the repressor derivative had lost its ability to bind operator specifically even though it could dimerize effectively. In similar studies, we demonstrated that an N-terminal portion of PENI with a molecular mass of 10 kDa derived by digestion with papain was able to bind operator specifically but with reduced affinity and had completely lost its ability to dimerize. These data suggest that the repressor has two functional and separable domains. The amino-terminal domain of the repressor is responsible for operator recognition, and the carboxyl-terminal domain is involved in subunit dimerization.
机译:青霉素酶阻遏物(PENI)与地衣芽孢杆菌中的青霉素酶基因(penP)的表达负相关,与位于penP启动子区内的操纵子结合。penI编码具有128个氨基酸的蛋白质。过滤器结合分析表明阻遏物的活性形式是二聚体。 PENI衍生物的遗传分析表明,阻遏物在N端附近带有6个氨基酸的缺失或在C端带有14个氨基酸的阻遏物在体内没有功能。广泛纯化在其N端区域内携带6个氨基酸缺失的阻遏物衍生物,并将其用于DNA足迹和亚基交联分析。这些研究的结果表明,即使阻遏物衍生物可以有效地二聚,它也失去了特异性结合操纵子的能力。在类似的研究中,我们证明了用木瓜蛋白酶消化而得的分子量为10 kDa的PENI的N端部分能够特异性结合操纵子,但亲和力降低,并且完全丧失了其二聚化能力。这些数据表明阻遏物具有两个功能域和可分离域。阻遏物的氨基末端结构域负责操纵子识别,而羧基末端结构域参与亚基二聚化。

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