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The lethal and mutagenic effects of nitrous acid (0,1 M NaNO2 in 0,1 M acetate buffer, pH 4.6) on prophage lambda cI857 ind- were studied in the wild-type cells of Escherichia coli and in 9 repair-deficient mutants: uvrA6, uvrA6 umuC36, uvrD3, uvrE502, polA1, recA13, lexA102, recF143 and xthA9. After treatment with HNO2, the prophage was heat-induced either immediately or after 90 min incubation in broth at 32 degrees C. The prophage survival after delayed induction was considerably higher than after immediate induction. The lethal action of HNO2 was highly expressed in uvrA- and uvrE- lysogens after delayed induction. The frequency of temperature-independent c mutants forming clear plaques at 32 degrees C reached 4% in the wild-type host after immediate induction, this value being 10-15% in uvrA, uvrA umuC, uvrD, uvrE, polA and xthA mutants, 0,8% in recF- lysogen and only 0,2-0,3% in recA and lexA mutants. Under these conditions, about 90% of c mutants are generated by recA+, lexA+-dependent repair mechanism (most probably, due to W-mutagenesis). After delayed induction, mutation frequency in the wild-type host declines considerably (down to 0,1%). Analogous phenomenon of mutation frequency decline was registered in uvrA, xthA, recF, polA, uvrE and uvrD lysogens. Under conditions of delayed induction, the frequency of HNO2-induced c mutations only slightly depends on the recA+ and lexA+ gene products and mutations are, apparently, fixed by replication.  相似文献   

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The mutagenic activity of the monofunctional alkylating agent ethylenimine (EI) was tested with the adenine-3 (ad-3) system in a two-component heterokaryon of Neurospora crassa. The results of forward-mutation experiments showed that EI is a potent mutagen in N. crassa.Genetic analysis of EI-induced ad-3 mutants showed that the frequencies of leakiness, allelic complementation, and non-polarized complementation patterns are similar to those of ad-3 mutants induced by other alkylating agents. It seems, therefore, that in addition to multilocus deletions (which occur at low a frequency), EI-induced mutations probably include base-pair substitutions, frameshift mutations, and other types of intragenic alterations.  相似文献   

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Mutation at the am locus of Neurospora crassa   总被引:7,自引:2,他引:5       下载免费PDF全文
J A Kinsey  B S Hung 《Genetics》1981,99(3-4):405-414
Forty-eight new mutations at the am locus of Neurospora crassa have been characterized. Nineteen mutations were induced by UV; of these, eight were missense, two were frameshifts, two were nonsense, three were deletions and four were unidentified. Twenty-nine mutations were induced with nitrous acid; of these, twenty-one were missense, three were frameshifts, one was nonsense, two were deletions and one was genetically unstable.  相似文献   

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Organization of the histidine-3 region of Neurospora   总被引:3,自引:0,他引:3  
Summary The histidine-3 region of Neurospora specifies the structure of three enzymes of the histidine biosynthetic pathway viz., PR-AMP 1,6-cyclohydrolase, PR-ATP pyrophosphohydrolase, and histidinol dehydrogenase. Point mutations in this region may either affect individual enzyme activities or all of the three activities simultaneously. Attempts have been made to fractionate the three enzymes in order to understand the organization of the his-3 region. Gel-filtration on Sephadex G-200 revealed a single peak of activity for pyrophosphohydrolase and dehydrogenase. The two enzymes also emerged as one peak on chromatography through a DEAE-cellulose column eluted with linear salt gradient. Sedimentation characteristics of cyclohydrolase, pyrophosphohydrolase, and dehydrogenase were identical on sucrose density-gradient centrifugation. The molecular weight of this aggregate was estimated to be about 140,000. Other enzymes of histidine biosynthesis could be readily separated by these methods. Furthermore, mutational events occurring at several points across the genetic map seem to influence the three activities simultaneously. These results suggest that the polypeptides coded by the his-3 region are organized into a functional aggregate or multi-enzyme complex. Analysis of existing four-point cross data indicates that recombination within his-3 region is polarized. This polarity, according to the model proposed by Bernstein (1964), is towards the centromere and proceeds in a direction opposite to translation as deduced from complementation.  相似文献   

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A new locus in the tryptophan pathway of Neurospora crassa   总被引:2,自引:0,他引:2  
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Summary The mutagenicity and mutagenic specificity of aflatoxin B1 and G1 were studied with the adenine-3 (ad-3) test system of Neurospora crassa. Aflatoxin B1 and G1 failed to show mutagenicity in resting conidia, but both agents were mutagenic in growing vegetative cultures. The frequencies of ad-3 mutants induced by aflatoxin B1 and G1 (40g/ml) were 70.7x10-6 survivors and 9.6x10-6 survivors, respectively. Since aflatoxin B1 gave a 177-fold increase over the spontaneous mutation frequency it is a rather potent mutagen, whereas aflatoxin G1 gave only a 24-fold increase and so is only moderately mutagenic.Genetic analyses of ad-3 mutants induced by aflatoxin B1 and G1 indicate that both agents induce a low frequency of multilocus deletions. The spectra of point mutations at the ad-3A and ad-3B loci induced by aflatoxin B1 and G1 are not distinguishable from each other. Hence both agents probably induce the same relative frequencies of genetic alterations. The frequencies of leakiness, allelic complementation, and classes of complementation patterns among the ad-3 mutants induced by both agents are higher than the frequencies among ICR-170-induced mutants and somewhat lower than those among NA- and AP-induced mutants. The results of reversion tests with NA, MNNG, and ICR-170 indicate that in addition to multilocus deletion, aflatoxin B1-induced ad-3 mutants consist of frameshifts, base-pair transitions, and possibly other types of intragenic alterations.  相似文献   

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Summary Thepyrimidine-3 locus ofNeurospora crassa specifies two enzyme activities, pyrimidine-specific carbamyl phosphate synthetase (CPSpyr) and aspartate transcarbamylase (ATC). ATC is translationally distal. CPSpyr, but not ATC, is subject to feedback inhibition by uridine triphosphate (UTP). To investigate the location of the feedback-specific region within the locus, inhibition of a number ofpyr-3 alleles by UTP was investigated. All CPS+ ATC- polar alleles, revertants of CPS- ATC- polar alleles, and 5-fluorouracil-resistant mutants had normal UTP response. The location of the feedback-specific region is in or close to the CPS-specific region.Supported by Science Research Council Grant B/RG/2981  相似文献   

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