A novel bacterial vector system for monitoring protein-protein interactions in the cAMP-dependent protein kinase complex

A bacterial expression vector is described for investigation of protein-protein interactions. Important features of the vector include partition of the cI repressor of bacteriophage λ into two functional domains separated by a multicloning site, and low level auto-regulated expression of human genes as C-terminal fusions to the DNA-binding domain of cI. Two different reporter systems have been employed; expression of either a suppressor tRNA or the alkaline phosphatase gene is dependent in both cases on the extent of repression of the major leftward promoter of lambda (λP_L). The cAMP-dependent protein kinase (PKA) has been used as a model protein complex because both homodimer and heterodimer interactions are known to occur and because cAMP acts as a modulator of these interactions. It has been shown that the product of the repressor gene with newly incorporated expressed polylinker restriction sites still functions as a repressor. Substitution of the dimerisation domain of the cI repressor with the regulatory subunit of PKA does not diminish the ability of a cI fusion protein to repress expression of the reporter gene from λP_L, indicating that the regulatory subunit of PKA dimerises the fusion protein in the Escherichia coli cytoplasm. Substitution instead with the catalytic subunit of PKA destroys the repression ability of cI, which is partially restored by separate expression of the regulatory subunit within the same cell. Complete restoration is achieved using a host E. coli strain which has lost its ability to synthesise cAMP and again this can be reversed by the addition of exogenous cAMP to these cells. Human PKA has been reconstituted in the E. coli cytoplasm, where all subunit interactions appear functional and respond as expected to the allosteric modulator cAMP.     

NRSE 与 NRSF 及其对神经元特异性基因表达的调控作用

神经限制性沉默元件 (NRSE) 是一段长度为 21~23 bp 的保守 DNA 序列,存在于许多神经元特异表达基因的转录调控区中,神经限制性沉默因子 (NRSF) 能特异性结合到 NRSE dsDNA 上,并通过其 N 端和 C 端阻遏结构域分别连接共阻遏蛋白 Sin3A/B 和 CoREST , Sin3A 招募 HDAC 对组蛋白进行去乙酰基化修饰, CoREST 则作为平台蛋白招募特异的“沉默组件”,以此维持基因沉默 . 最近的研究显示, NRSE dsRNA 能在转录水平与 NRSF 蛋白直接作用,而不是作为 siRNA 或 miRNA 在转录后水平启动神经元特异性基因的表达 .