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Contacts between Escherichia coli RNA polymerase and an early promoter of phage T7. 总被引:35,自引:1,他引:35
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U Siebenlist W Gilbert 《Proceedings of the National Academy of Sciences of the United States of America》1980,77(1):122-126
Specific contacts between the Escherichia coli RNA polymerase (nucleosidetriphosphate:RNA nucleotidyl-transferase, EC2.7.7.6) and the phosphates and purine bases of the A3 promoter of phage T7 cluster into three regions located approximately 10, 16, and 35 base pairs before RNA initiation site. Two of these contain nucleotide sequences that are fairly conserved among many promoters, known as the "Pribnow box" and "-35 region" homologies; the third, just upstream from the Pribnow box, is not conserved. The polymerase binds preferentially to the coding strand and for the most part touches only one face of the DNA helix. 相似文献
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Mutational analysis of an archaebacterial promoter: essential role of a TATA box for transcription efficiency and start-site selection in vitro. 总被引:31,自引:9,他引:31
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W D Reiter U Hüdepohl W Zillig 《Proceedings of the National Academy of Sciences of the United States of America》1990,87(24):9509-9513
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Point mutations and DNA rearrangements 5'' to the inducible qa-2 gene of Neurospora allow activator protein-independent transcription. 总被引:5,自引:2,他引:5
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R F Geever M E Case B M Tyler F Buxton N H Giles 《Proceedings of the National Academy of Sciences of the United States of America》1983,80(23):7298-7302
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J E Stefano J D Gralla 《Proceedings of the National Academy of Sciences of the United States of America》1982,79(4):1069-1072
Mutations have been constructed that delete either one or two base pairs near position -19 in the lac ps promoter. Deletion of either of two adjacent base pairs increases the rates of open complex formation by nearly on order of magnitude. Two promoters that have different single-base deletions are indistinguishable by either their rates of open complex formation or stability of the open complexes once formed. However, simultaneous deletion of both base pairs produces a promoter that forms complexes at a rate similar to that of the unmodified DNA sequence. The maximal rate of open complex formation is achieved at a spacer length of 17 base pairs, the most frequently occurring spacer length among promoters. These results suggest that the spacing between the two strongly conserved regions of sequence homology is an important determinant of the rate of open complex formation. A model is suggested that proposes that three important promoter elements, the -10 region, the -35 region, and the spacer region, act simultaneously to facilitate open complex formation by RNA polymerase. 相似文献
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Nucleotide sequence of an RNA polymerase binding site at an early T7 promoter. 总被引:21,自引:2,他引:21
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D Pribnow 《Proceedings of the National Academy of Sciences of the United States of America》1975,72(3):784-788
Escherichia coli RNA polymerase (EC 2.7.7.6), bound in a tight complex at an early T7 promoter, protects 41 to 43 base pairs of DNA from digestion by DNase. I. The protected DNA fragment contains both the binding site for RNA polymerase and the mRNA initiation point for the promoter. The sequence of the DNA fragment and the sequence of the mRNA that it codes for are presented here. A seven-base-pair sequence, apparently common to all promoters, is implicated in the formation of a tight binary complex with RNA polymerase. 相似文献