EFFECTS OF MUTATIONS OF THE BULGED NUCLEOTIDE IN THE CONSERVED P7 PAIRING ELEMENT OF THE PHAGE-T4 TD INTRON ON RIBOZYME FUNCTION

被引:29
作者
SCHROEDER, R
VONAHSEN, U
BELFORT, M
机构
[1] NEW YORK STATE DEPT HLTH,WADSWORTH CTR LABS & RES,EMPIRE STATE PLAZA,POB 509,ALBANY,NY 12201
[2] SUNY ALBANY,SCH PUBL HLTH,ALBANY,NY 12201
[3] UNIV VIENNA,INST MIKROBIOL & GENET,A-1090 VIENNA,AUSTRIA
关键词
D O I
10.1021/bi00227a018
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 P7 element of group I introns contains a semiconserved "bulged" nucleotide, a C in group IA introns (nt 870 in the td intron) and an A in group IB introns [Cech, T. R. (1988) Gene 73, 259-271]. Variants U870, G870, and A870, isolated by a combination of in vitro and in vivo genetic strategies, indicate that C and A at position 870 are consistent with splicing whereas U and G are not. Although mutants G870 and U870 could be activated in vitro by increasing the Mg2+ concentration, their K(m) for GTP at pH 7 was 20-100-fold elevated, and they were unable to undergo site-specific hydrolysis. The dependence of the mutants on high guanosine concentrations could be substantially overcome by an increase in pH, suggesting that a tautomeric change, which makes U and G mimic C and A, is responsible for restoring function. In contrast to the striking K(m) effect, V(max) for the mutants differed by less than a factor of 2 from the wild type. Furthermore, streptomycin, an aminoglycoside antibiotic that competes with guanosine for its binding site, inhibited splicing of the U870 and G870 constructs at least as well as of the C870 and A870 variants, indicating that the guanosine-binding site of the mutants is proficient at interacting with a guanidino group. While our experiments argue against a hydrogen-bonding interaction between the C6-O of the cofactor and C4-NH2 of the bulged nucleotide, they are consistent with other models in which the C4-NH2 and/or N3 groups of the bulged C are involved in establishing an active ribozyme.
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页码:3295 / 3303
页数:9
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