Christie Gail E, Anders Douglas L, McAlister Victor, Goodwin Tina S, Julien Bryan, Calendar Richard
Department of Microbiology and Immunology, Virginia Commonwealth University, Richmond, Virginia, USA.
J Bacteriol. 2003 Aug;185(15):4609-14. doi: 10.1128/JB.185.15.4609-4614.2003.
We have carried out a mutational scan of the upstream region of the bacteriophage P2 FETUD late operon promoter, P(F), which spans an element of hyphenated dyad symmetry that is conserved among all six of the P2 and P4 late promoters. All mutants were assayed for activation by P4 delta in vivo, by using a lacZ reporter plasmid, and a subset of mutants was assayed in vitro for delta binding. The results confirm the critical role of the three complementary nucleotides in each half site of the upstream element for transcription factor binding and for activation of transcription. A trinucleotide DNA recognition site is consistent with a model in which these transcription factors bind via a zinc finger motif. The mutational scan also led to identification of the -35 region of the promoter. Introduction of a sigma(70) -35 consensus sequence resulted in increased constitutive expression, which could be further stimulated by delta. These results indicate that activator binding to the upstream region of P2 late promoters compensates in part for poor sigma(70) contacts and helps to recruit RNA polymerase holoenzyme.
我们对噬菌体P2 FETUD晚期操纵子启动子P(F)的上游区域进行了突变扫描,该区域跨越一个具有连字符的二元对称元件,在所有六个P2和P4晚期启动子中都是保守的。使用lacZ报告质粒,对所有突变体进行了体内P4δ激活检测,并且对一部分突变体进行了体外δ结合检测。结果证实了上游元件每个半位点中的三个互补核苷酸对于转录因子结合和转录激活的关键作用。三核苷酸DNA识别位点与这些转录因子通过锌指基序结合的模型一致。突变扫描还导致了启动子-35区域的鉴定。引入σ(70) -35共有序列导致组成型表达增加,这可以被δ进一步刺激。这些结果表明,激活剂与P2晚期启动子上游区域的结合部分补偿了σ(70)接触不良的问题,并有助于募集RNA聚合酶全酶。
