学术探索
学术期刊
新闻热点
数据分析
智能评审

SPECIAL PEPTIDYL-TRANSFER-RNA MOLECULES CAN PROMOTE TRANSLATIONAL FRAMESHIFTING WITHOUT SLIPPAGE

被引:50
作者
VIMALADITHAN, A [1 ]
FARABAUGH, PJ [1 ]
机构
[1] UNIV MARYLAND, DEPT BIOL SCI, CATONSVILLE, MD 21228 USA
来源
MOLECULAR AND CELLULAR BIOLOGY | 1994年 / 14卷 / 12期
关键词
D O I
10.1128/MCB.14.12.8107
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
Recently we described an unusual programmed +1 frameshift event in yeast retrotransposon Ty3. Frameshifting depends on the presence of peptidyl-tRNA(CGC)(Ala) on the GCG codon in the ribosomal P site and on a translational pause stimulated by the slowly decoded AGU codon. Frameshifting occurs on the sequence GCG-AGU-U by out-of-frame binding of a valyl-tRNA to GUU without slippage of peptidyl-tRNA(CGC)(Ala). This mechanism challenges the conventional understanding that frameshift efficiency must correlate with the ability of mRNA-bound tRNA to slip between cognate or near-cognate codons. Though frameshifting does not require slippery tRNAs, it does require special peptidyl-tRNAs. We show that overproducing second isoacceptor whose anticodon had been changed to CGC eliminated frameshifting; peptidyl-tRNA(CGC)(Ala) must have a special capacity to induce +1 frameshifting in the adjacent ribosomal A site. In order to identify other special peptidyl-tRNAs, we tested the ability of each of the other 63 codons to replace GCG in the P site. We found no correlation between the ability to stimulate +1 frameshifting and the ability of the cognate tRNA to slip on the mRNA-several codons predicted to slip efficiently do not stimulate frameshifting, while several predicted not to slip do stimulate frameshifting. By inducing a severe translational pause, we identified eight tRNAs capable of inducing measurable +1 frameshifting, only four of which are predicted to slip on the mRNA. We conclude that in Saccharomyces cerevisiae, special peptidyl-tRNAs can induce frameshifting dependent on some characteristic(s) other than the ability to slip on the mRNA.
引用
收藏
页码:8107 / 8116
页数:10
相关论文
共 59 条
[11]   EXPRESSION OF PEPTIDE-CHAIN RELEASE FACTOR-II REQUIRES HIGH-EFFICIENCY FRAMESHIFT [J].
CRAIGEN, WJ ;
CASKEY, CT .
NATURE, 1986, 322 (6076) :273-275
[12]   READING FRAME SELECTION AND TRANSFER-RNA ANTICODON LOOP STACKING [J].
CURRAN, JF ;
YARUS, M .
SCIENCE, 1987, 238 (4833) :1545-1550
[13]   USE OF TRANSFER-RNA SUPPRESSORS TO PROBE REGULATION OF ESCHERICHIA-COLI RELEASE FACTOR-II [J].
CURRAN, JF ;
YARUS, M .
JOURNAL OF MOLECULAR BIOLOGY, 1988, 203 (01) :75-83
[14]   ANALYSIS OF EFFECTS OF TRANSFER-RNA - MESSAGE STABILITY ON FRAMESHIFT FREQUENCY AT THE ESCHERICHIA-COLI RF2 PROGRAMMED FRAMESHIFT SITE [J].
CURRAN, JF .
NUCLEIC ACIDS RESEARCH, 1993, 21 (08) :1837-1843
[15]   A -1 RIBOSOMAL FRAMESHIFT IN A DOUBLE-STRANDED-RNA VIRUS OF YEAST FORMS A GAG POL FUSION PROTEIN [J].
DINMAN, JD ;
ICHO, T ;
WICKNER, RB .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1991, 88 (01) :174-178
[16]   FRAMESHIFT AUTOREGULATION IN THE GENE FOR ESCHERICHIA-COLI RELEASE FACTOR-II - PARTLY FUNCTIONAL MUTANTS RESULT IN FRAMESHIFT ENHANCEMENT [J].
DONLY, BC ;
EDGAR, CD ;
ADAMSKI, FM ;
TATE, WP .
NUCLEIC ACIDS RESEARCH, 1990, 18 (22) :6517-6522
[17]   HOW MANY EF-TU MOLECULES PARTICIPATE IN AMINOACYL-TRANSFER-RNA BINDING AND PEPTIDE-BOND FORMATION IN ESCHERICHIA-COLI TRANSLATION [J].
EHRENBERG, M ;
ROJAS, AM ;
WEISER, J ;
KURLAND, CG .
JOURNAL OF MOLECULAR BIOLOGY, 1990, 211 (04) :739-749
[18]   ENHANCER AND SILENCER-LIKE SITES WITHIN THE TRANSCRIBED PORTION OF A TY2 TRANSPOSABLE ELEMENT OF SACCHAROMYCES-CEREVISIAE [J].
FARABAUGH, P ;
LIAO, XB ;
BELCOURT, M ;
ZHAO, H ;
KAPAKOS, J ;
CLARE, J .
MOLECULAR AND CELLULAR BIOLOGY, 1989, 9 (11) :4824-4834
[19]   3 DOWNSTREAM SITES REPRESS TRANSCRIPTION OF A TY2 RETROTRANSPOSON IN SACCHAROMYCES-CEREVISIAE [J].
FARABAUGH, PJ ;
VIMALADITHAN, A ;
TURKEL, S ;
JOHNSON, R ;
ZHAO, H .
MOLECULAR AND CELLULAR BIOLOGY, 1993, 13 (04) :2081-2090
[20]   ALTERNATIVE READINGS OF THE GENETIC-CODE [J].
FARABAUGH, PJ .
CELL, 1993, 74 (04) :591-596
123456