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Literature DB >> 2849240

Q-mediated late gene transcription of bacteriophage lambda: RNA start point and RNase III processing sites in vivo.

D L Daniels¹, M N Subbarao, F R Blattner, H A Lozeron.

Abstract

The location of the RNA start point of in vivo Q-activated late gene RNA of bacteriophage lambda has been determined to be identical to the start point of in vitro 6 S RNA. The 6 S RNA is made early in infection and is efficiently antiterminated by Q. Two RNase III cut sites are located within Q-dependent RNA sequences, 209 and 270 bp from the beginning of the late transcript, and lie on the stem of an inverted repeat which has features in common with previously described RNase III processing sites. This is the third example of RNase III cut sites immediately downstream of transcription termination points in lambda, the others being antiterminated N gene mRNA and int gene mRNA.

Entities: Disease Species

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Year: 1988 PMID： 2849240

Source DB: PubMed Journal: Virology ISSN： 0042-6822 Impact factor: 3.616

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Cited

11 in total

Review 1. Bacteriophage lysis: mechanism and regulation.

Authors: R Young
Journal: Microbiol Rev Date: 1992-09

2. The global regulator RNase III modulates translation repression by the transcription elongation factor N.

Authors: Helen R Wilson; Daiguan Yu; Howard K Peters; Jian-guang Zhou; Donald L Court
Journal: EMBO J Date: 2002-08-01 Impact factor: 11.598

3. The cleavage specificity of RNase III.

Authors: L Krinke; D L Wulff
Journal: Nucleic Acids Res Date: 1990-08-25 Impact factor: 16.971

4. A conserved sequence element in ribonuclease III processing signals is not required for accurate in vitro enzymatic cleavage.

Authors: B S Chelladurai; H Li; A W Nicholson
Journal: Nucleic Acids Res Date: 1991-04-25 Impact factor: 16.971

9. Cleavages in the 5' region of the ompA and bla mRNA control stability: studies with an E. coli mutant altering mRNA stability and a novel endoribonuclease.

Authors: U Lundberg; A von Gabain; O Melefors
Journal: EMBO J Date: 1990-09 Impact factor: 11.598

10. Autoregulation of RNase III operon by mRNA processing.

Authors: J C Bardwell; P Régnier; S M Chen; Y Nakamura; M Grunberg-Manago; D L Court
Journal: EMBO J Date: 1989-11 Impact factor: 11.598

Q-mediated late gene transcription of bacteriophage lambda: RNA start point and RNase III processing sites in vivo.

Review 1. Bacteriophage lysis: mechanism and regulation.

2. The global regulator RNase III modulates translation repression by the transcription elongation factor N.

3. The cleavage specificity of RNase III.

4. A conserved sequence element in ribonuclease III processing signals is not required for accurate in vitro enzymatic cleavage.

5. Rescue of the RNA phage genome from RNase III cleavage.

6. S gene expression and the timing of lysis by bacteriophage lambda.

7. Analysis of mRNA decay and rRNA processing in Escherichia coli multiple mutants carrying a deletion in RNase III.

8. Role for a phage promoter in Shiga toxin 2 expression from a pathogenic Escherichia coli strain.

9. Cleavages in the 5' region of the ompA and bla mRNA control stability: studies with an E. coli mutant altering mRNA stability and a novel endoribonuclease.

10. Autoregulation of RNase III operon by mRNA processing.