STEP-ARREST MUTANTS OF PHAGE MU-TRANSPOSASE - IMPLICATIONS IN DNA-PROTEIN ASSEMBLY, MU-END CLEAVAGE, AND STRAND TRANSFER

被引：57

作者：

KIM, K ^{[1
]}

NAMGOONG, SY ^{[1
]}

JAYARAM, M ^{[1
]}

HARSHEY, RM ^{[1
]}

机构：

[1] UNIV TEXAS,DEPT MICROBIOL,AUSTIN,TX 78712

来源：

JOURNAL OF BIOLOGICAL CHEMISTRY | 1995年 / 270卷 / 03期

关键词：

D O I：

10.1074/jbc.270.3.1472

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

We describe the isolation and characterization of Mu A variants arrested at specific steps of transposition. Mutations at 13 residues within the Mu A protein were analyzed for precise excision of Mu DNA in vivo. A subset of the defective variants (altered at Asp(269), Asp(294), Gly(348), and Glu(392)) were tested in specific steps of transposition in vitro. It is possible that at least some residues of the Asp(269)-Asp(294)-Glu(392) triad may have functional similarities to those of the conserved Asp-Asp-Glu motif found in several transposases and retroviral integrases. Mu A(D269V) is defective in high-order DNA-protein assembly, Mu end cleavage, and strand transfer. The assembly defect, but not the catalytic defect, can be overcome by precleavage of Mu ends, Mu A(E392A) can assemble the synaptic complex, but cannot cleave Mu ends, A mutation of Gly(348) to aspartic acid within Mu A permits the uncoupling of cleavage and strand transfer activities. This mutant is completely defective in synaptic assembly and Mu end cleavage in presence of Mg2+. The assembly defect is alleviated by replacing Mg2+ with Ca2+. Some Mu end cleavage is observed with this mutant in the presence of Mn2+. When presented with precleaved Mu ends, Mu A(G348D) exhibits efficient strand transfer activity.

引用

页码：1472 / 1479

页数：8

共 41 条

[1] DIVISION-OF-LABOR AMONG MONOMERS WITHIN THE MU-TRANSPOSASE TETRAMER
BAKER, TA
MIZUUCHI, M
SAVILAHTI, H
MIZUUCHI, K
[J]. CELL, 1993, 74 (04) : 723 - 733
[2] MUB PROTEIN ALLOSTERICALLY ACTIVATES STRAND TRANSFER BY THE TRANSPOSASE OF PHAGE-MU
BAKER, TA
MIZUUCHI, M
MIZUUCHI, K
[J]. CELL, 1991, 65 (06) : 1003 - 1013
[3] BAKER TA, 1994, P NATL ACAD SCI USA, V91, P6645
[4] Barik S, 1993, Methods Mol Biol, V15, P277, DOI 10.1385/0-89603-244-2:277
[5] STRUCTURAL BASIS FOR THE 3'-5' EXONUCLEASE ACTIVITY OF ESCHERICHIA-COLI DNA-POLYMERASE-I - A 2 METAL-ION MECHANISM
BEESE, LS
STEITZ, TA
[J]. EMBO JOURNAL, 1991, 10 (01) : 25 - 33
[6] FUNCTIONAL DOMAINS OF BACTERIOPHAGE-MU TRANSPOSASE - PROPERTIES OF C-TERMINAL DELETIONS
BETERMIER, M
ALAZARD, R
LEFRERE, V
CHANDLER, M
[J]. MOLECULAR MICROBIOLOGY, 1989, 3 (09) : 1159 - 1171
[7] TRANSPOSITION OF GAMMA-PLACMUS IS MEDIATED IN THE A-PROTEIN ALTERED AT ITS CARBOXY-TERMINAL END
BREMER, E
SILHAVY, TJ
WEINSTOCK, GM
[J]. GENE, 1988, 71 (01) : 177 - 186
[8] REVERSAL OF MUTATOR PHAGE MU-INTEGRATION
BUKHARI, AI
[J]. JOURNAL OF MOLECULAR BIOLOGY, 1975, 96 (01) : 87 - &
[9] DNA CLEAVAGE IN TRANS BY THE ACTIVE-SITE TYROSINE DURING FLP RECOMBINATION - SWITCHING PROTEIN PARTNERS BEFORE EXCHANGING STRANDS
CHEN, JW
LEE, J
JAYARAM, M
[J]. CELL, 1992, 69 (04) : 647 - 658
[10] THE 3'-5' EXONUCLEASE OF DNA-POLYMERASE-I OF ESCHERICHIA-COLI - CONTRIBUTION OF EACH AMINO-ACID AT THE ACTIVE-SITE TO THE REACTION
DERBYSHIRE, V
GRINDLEY, NDF
JOYCE, CM
[J]. EMBO JOURNAL, 1991, 10 (01) : 17 - 24

← 1 2 3 4 5 →