pT181质粒起始蛋白RepC的失活形式RepC/C*的体外抑制活性
In vitro inhibitory activity of RepC/C*, the inactivated form of the pT181 plasmid initiation protein, RepC.
作者信息
Jin R, Rasooly A, Novick R P
机构信息
Molecular Pathogenesis Program, Skirball Institute, New York University School of Medicine, New York, New York 10016, USA.
出版信息
J Bacteriol. 1997 Jan;179(1):141-7. doi: 10.1128/jb.179.1.141-147.1997.
pT181 is a Staphylococcus aureus rolling circle plasmid that regulates its replication by controlling the synthesis of its dimeric initiator protein RepC/C and by inactivating the protein following its use in replication (A. Rasooly and R. P. Novick, Science 262:1048-1050, 1993). This inactivation consists of the addition of an oligonucleotide, representing several nucleotides immediately 3' to the initiation nick site, to the active site tyrosine of one of the two subunits, generating a heterodimer, RepC/C*. Previous results suggested that the inactive form was metabolically stable and was present at a much higher level than the active form (A. Rasooly and R. P. Novick, Science 262:1048-1050, 1993). In the present study we have measured total RepC antigen as a function of plasmid copy number and have analyzed the interaction of the two forms. We find that pT181-containing staphylococci contain approximately one RepC dimer per plasmid copy over a 50-fold range of copy numbers. This is consistent with previous measurements of the rate of RepC synthesis, which suggested that one RepC dimer is synthesized per replication event (J. Bargonetti, P.-Z. Wang and R. P. Novick, EMBO J. 12:3659-3667, 1993). The RepC/C* heterodimer, which is inactive for replication, is a competitive inhibitor of the replication and the topoisomerase-like and cruciform-enhancing activities of the native protein. These results suggest that the inactive form may have a specific regulatory role in vivo. Since the known plasmid-determined controls, which maintain a constant plasmid copy number, are designed to ensure the synthesis of one RepC/C dimer per plasmid replication event, it is difficult to envision any role for yet another negative regulator of replication. Conceivably, under conditions where the initiator is overproduced, such as in the absence of the normal antisense regulation of initiator production, RepC/C* could serve as a fail-safe means of preventing autocatalytic replication.
pT181是一种金黄色葡萄球菌滚环质粒,它通过控制其二聚体起始蛋白RepC/C的合成以及在复制过程中使用该蛋白后使其失活来调节自身复制(A. Rasooly和R. P. Novick,《科学》262:1048 - 1050,1993年)。这种失活包括在两个亚基之一的活性位点酪氨酸上添加一个寡核苷酸,该寡核苷酸代表紧邻起始切口位点3'端的几个核苷酸,从而产生异二聚体RepC/C*。先前的结果表明,无活性形式在代谢上是稳定的,并且其存在水平比活性形式高得多(A. Rasooly和R. P. Novick,《科学》262:1048 - 1050,1993年)。在本研究中,我们测量了总RepC抗原作为质粒拷贝数的函数,并分析了两种形式之间的相互作用。我们发现,在拷贝数范围达50倍的情况下,含pT181的葡萄球菌每个质粒拷贝大约含有一个RepC二聚体。这与先前对RepC合成速率的测量结果一致,先前的测量结果表明每个复制事件合成一个RepC二聚体(J. Bargonetti、P.-Z. Wang和R. P. Novick,《欧洲分子生物学组织杂志》12:3659 - 3667,1993年)。对复制无活性的RepC/C异二聚体是天然蛋白复制、拓扑异构酶样活性和十字形增强活性的竞争性抑制剂。这些结果表明,无活性形式在体内可能具有特定的调节作用。由于已知的维持恒定质粒拷贝数的质粒决定的控制机制旨在确保每个质粒复制事件合成一个RepC/C二聚体,因此很难设想另一种复制负调节因子会有任何作用。可以想象,在起始蛋白过量产生的条件下,例如在缺乏起始蛋白产生的正常反义调节的情况下,RepC/C可以作为防止自催化复制的一种保险措施。
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