Bernard S. Strauss scite author profile

M13 DNA containing 20-30 apurinic/apyrimidinic (AP) sites per intact circular molecule was prepared by growing phage on an ung- dut- Escherichia coli mutant and treating the DNA with uracil N-glycosylase. AP sites obstruct in vitro DNA synthesis catalyzed by E. coli pol I. The position at which termination of synthesis occurs was determined for four enzymes. T4 DNA polymerase terminates one nucleotide before putative AP sites. DNA pol I, AMV reverse transcriptase, and DNA polymerase alpha terminate synthesis either before or at the site of an AP lesion depending on the particular sequence. We determined the identity of the nucleotide inserted opposite an AP site by synthesizing up to the lesion in a first-stage reaction using T4 DNA polymerase and then determining elongation in a second stage. Purines are inserted opposite AP sites more readily than pyrimidines, and dATP is more efficient than dGTP in promoting such elongation. The DNA-dependent conversion of dNTP to dNMP was determined in mixtures of all four dNTP's by using AP DNA. The production of dAMP from dATP occurs most readily. We conclude that there is an inherent specificity for the incorporation of adenine nucleotides opposite AP sites in this in vitro system. Insofar as the model system reflects in vivo mutational events, our data suggest that depurination should produce transversions and depyrimidination should produce transitions.

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The ‘A rule’ of mutagen specificity: A consequence of DNA polymerase bypass of non‐instructional lesions?

Strauss

1991

BioEssays

251

152

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The replicative bypass of lesions in DNA and the induction of mutations by agents which react with DNA to produce damaged bases can be understood on the basis of a simple kinetic model. Bypass can be analyzed by separately considering three processes: a) addition of a base opposite a lesion, b) a proofreading excision process, and c) a rate limiting elongation step. Adenine nucleotides are preferentially added opposite many lesions making it possible to predict mutational specificity. Replicative bypass (translesion synthesis) is dependent on modulation of proofreading exonuclease activity but loss of exonuclease activity alone is not sufficient to ensure bypass. Frameshift mutation is the result of the failure of translesion synthesis accompanied by rearrangement of the template, particularly at repetitive sites.

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The role of DNA polymerase in base substitution mutagenesis on non-instructional templates

Strauss¹,

Rabkin²,

Sagher³

et al. 1982

Biochimie

158

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Sites of inhibition of in vitro DNA synthesis in carcinogen- and UV-treated Φ174 DNA

Moore¹,

Strauss²

1979

Nature

188

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The “A” rule revisited: polymerases as determinants of mutational specificity

Strauss¹

2002

DNA Repair

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The possible role of recombination in the infection of competent Bacillus subtilis by bacteriophage deoxyribonucleic acid

Okubo¹,

Strauss²,

Stodolsky³

1964

Virology

168

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Role of thedinBGene Product in Spontaneous Mutation inEscherichia coliwith an Impaired Replicative Polymerase

et al. 2000

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We isolated several new mutator mutations of the Escherichia coli replicative polymerase dnaE subunit alpha and used them and a previously reported dnaE mutation to study spontaneous frameshift and base substitution mutations. Two of these dnaE strains produce many more mutants when grown on rich (Luria-Bertani) than on minimal medium. A differential effect of the medium was not observed when these dnaE mutations were combined with a mismatch repair mutation. The selection scheme for the dnaE mutations required that they be able to complement a temperature-sensitive strain. However, the ability to complement is not related to the mutator effect for at least one of the mutants. Comparison of the mutation rates for frameshift and base substitution mutations in mutS and dnaE mutS strains suggests that the mismatch repair proteins respond differently to the two types of change. Deletion of dinB from both chromosome and plasmid resulted in a fourto fivefold decrease in the rate of frameshift and base substitution mutations in a dnaE mutS double mutant background. This reduction indicates that most mistakes in replication occur as a result of the action of the auxiliary rather than the replicative polymerase in this dnaE mutant. Deletion of dinB from strains carrying a wild-type dnaE had a measurable effect, suggesting that a fraction of spontaneous mutations occur as a result of dinB polymerase action even in cells with a normal replicative polymerase.Mutation is a characteristic of all living systems and provides the material for natural selection (43, 48). However, most mutations are deleterious, and organisms have evolved mechanisms to protect themselves from excessive mutation rates. These protective mechanisms recognize and correct mismatches that have occurred in DNA as a result of replication or spontaneous deamination and recognize and remove potentially mutagenic changes that have occurred as a result of the reaction of the DNA with endogenous or exogenous mutagens (21). The activity of these repair systems can be modulated, and one method of increasing the rate of mutations either permanently or transiently is to decrease the activity of the repair systems, e.g., mismatch repair (14). It has generally been assumed that the interaction of the error repair systems with the natural error rate of the replicative DNA polymerases satisfactorily accounts for mutation rates and their modulation (7). However, among the characteristics of biological systems are their complexity and the multilevels of control that they employ. Regulation, for example, is characterized by both accelerating and inhibiting or braking features, and this principle can be seen in systems as diverse as the regulation of the rate of the heartbeat in vertebrates (38) and the regulation of lactose utilization in bacteria (31). The recent discoveries of DNA polymerases which seem designed to produce a high frequency of errors should therefore not be viewed with surprise, but rather as another illustration of the redundancy with which organisms m...

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