PROTEIN SPLICING REMOVES INTERVENING SEQUENCES IN AN ARCHAEA DNA-POLYMERASE

被引：115

作者：

HODGES, RA ^{[1
]}

PERLER, FB ^{[1
]}

NOREN, CJ ^{[1
]}

JACK, WE ^{[1
]}

机构：

[1] NEW ENGLAND BIOLABS INC,32 TOZER ROAD,BEVERLY,MA 01915

来源：

NUCLEIC ACIDS RESEARCH | 1992年 / 20卷 / 23期

关键词：

D O I：

10.1093/nar/20.23.6153

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：

The Vent DNA polymerase gene from Thermococcus litoralis contains two in-frame insertions that must be spliced out to form the mature polymerase. Primer extension and cDNA PCR revealed no evidence of spliced RNA to account for this editing. In contrast, pulse-chase analysis indicated that expression constructs lacking the first insertion produced a protein precursor in Escherichia coli that was processed post-translationally to form polymerase and I-TliI, the endonuclease protein that is the product of the second insertion. At least one intermediate, which migrated more slowly than the precursor and may be branched, was also detected. Amino acid substitutions at the splice junction slowed or blocked the protein splicing reaction. Processing occurs in several heterologous systems, indicating either self-splicing or ubiquitous splicing factors. Processing occurs in a mutant lacking I-TliI endonuclease activity, establishing the independence of splicing and endonuclease activities.

引用

页码：6153 / 6157

页数：5

共 23 条

[1] BELFORT M, 1990, ANNU REV GENET, V24, P363
[2] SELF-SPLICING OF GROUP-I INTRONS
CECH, TR
[J]. ANNUAL REVIEW OF BIOCHEMISTRY, 1990, 59 : 543 - 568
[3] CHOMCZYNSKI P, 1987, ANAL BIOCHEM, V162, P156, DOI 10.1016/0003-2697(87)90021-2
[4] ACTIVE-SITE MUTANTS OF BETA-LACTAMASE - USE OF AN INACTIVE DOUBLE MUTANT TO STUDY REQUIREMENTS FOR CATALYSIS
DALBADIEMCFARLAND, G
NEITZEL, JJ
RICHARDS, JH
[J]. BIOCHEMISTRY, 1986, 25 (02) : 332 - 338
[5] PROTEIN SPLICING IN THE MATURATION OF MYCOBACTERIUM-TUBERCULOSIS RECA PROTEIN - A MECHANISM FOR TOLERATING A NOVEL CLASS OF INTERVENING SEQUENCE
DAVIS, EO
JENNER, PJ
BROOKS, PC
COLSTON, MJ
SEDGWICK, SG
[J]. CELL, 1992, 71 (02) : 201 - 210
[6] NOVEL STRUCTURE OF THE RECA LOCUS OF MYCOBACTERIUM-TUBERCULOSIS IMPLIES PROCESSING OF THE GENE-PRODUCT
DAVIS, EO
SEDGWICK, SG
COLSTON, MJ
[J]. JOURNAL OF BACTERIOLOGY, 1991, 173 (18) : 5653 - 5662
[7] FERSHT A, 1977, ENZYME STRUCTURE MEC, P303
[8] RAPID PRODUCTION OF FULL-LENGTH CDNAS FROM RARE TRANSCRIPTS - AMPLIFICATION USING A SINGLE GENE-SPECIFIC OLIGONUCLEOTIDE PRIMER
FROHMAN, MA
DUSH, MK
MARTIN, GR
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1988, 85 (23) : 8998 - 9002
[9] THE ESCHERICHIA-COLI DNAY GENE ENDCODES AN ARGININE TRANSFER-RNA
GARCIA, GM
MAR, PK
MULLIN, DA
WALKER, JR
PRATHER, NE
[J]. CELL, 1986, 45 (03) : 453 - 459
[10] HOMING OF A DNA ENDONUCLEASE GENE BY MEIOTIC GENE CONVERSION IN SACCHAROMYCES-CEREVISIAE
GIMBLE, FS
THORNER, J
[J]. NATURE, 1992, 357 (6376) : 301 - 306

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