Role of error-prone DNA polymerases in spontaneous mutagenesis in <i>Caulobacter crescentus</i>

Valencia, Alexy O.; Braz, Vânia S.; Magalhães, Magna; Galhardo, Rodrigo S.

doi:10.1590/1678-4685-GMB-2018-0283

Alexy O. Valencia

Universidade de São Paulo, Instituto de Ciências Biomédicas, Departamento de Microbiologia, São Paulo, SP, Brazil.

http://orcid.org/0000-0001-9074-6823

Vânia S. Braz

Universidade de São Paulo, Instituto de Ciências Biomédicas, Departamento de Microbiologia, São Paulo, SP, Brazil.

Magna Magalhães

Universidade de São Paulo, Instituto de Ciências Biomédicas, Departamento de Microbiologia, São Paulo, SP, Brazil.

Rodrigo S. Galhardo Send correspondence to Rodrigo S. Galhardo. Universidade de São Paulo, Instituto de Ciências Biomédicas, Departamento de Microbiologia, Butantã, São Paulo, SP, Brazil. E-mail: rgalhard@usp.br.

Universidade de São Paulo, Instituto de Ciências Biomédicas, Departamento de Microbiologia, São Paulo, SP, Brazil.

http://orcid.org/0000-0002-5686-9704

Send correspondence to Rodrigo S. Galhardo. Universidade de São Paulo, Instituto de Ciências Biomédicas, Departamento de Microbiologia, Butantã, São Paulo, SP, Brazil. E-mail: rgalhard@usp.br.

Figures (5)
Tables (1)

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Figure 1
Rationale of the xylbla marker. The xylX gene in the xyl operon has been replaced by blaA. Nevertheless, repression by XylR in the absence of xylose renders cells phenotypically AmpS. Cells can become phenotypically AmpR by loss of function mutations (M) in xylR, or by mutations in the xylR operator inside PxylX.

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Figure 2
TetR and AmpR mutation rates. TetR mutation rates were determined using 66 cultures from 6 independent experiments. AmpR mutation rates were determined using 55 cultures from 5 independent experiments. Both the parental strains containing the cItet and xylbla markers (wt) and their dinB and imuC derivatives were analyzed. Mutation rates and 95% confidence intervals (represented by the error bars) were calculated using the MSS-MLE (Ma-Sandri-Sarkar Maximum Likelihood Estimator).

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Figure 3
Distribution of the different base substitutions in cI in wt, dinB and imuC strains. Results are shown for NA1000 strain (wt) and mutant strains (dinB and imuC). n indicates the number of mutants analyzed in each strain. The different base substitutions are indicated. Del 1 bp: 1 bp deletions. Ins 1 bp: 1 bp insertions. Ins 21 bp: 21 bp insertion detected in the wt strain.

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Figure 4
Distribution of the different base substitutions in xylR in wt, dinB and imuC strains. The different base substitutions are indicated. Del 1 bp: 1 bp deletions. Ins 1 bp: 1 bp insertions not located in the hotspot. Ins 1 bp hotspot: 1 bp insertions located in the hotspot. Small dels: 2-8 bp deletions. ME ins: insertion of mobile elements. n indicates the number of mutants analyzed in each strain.

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Figure 5
PxylX mutations. (A) Distribution of the different base substitutions in PxylX in wt (parental strain), dinB and imuC strains. The different base substitutions are indicated. n indicates the number of mutants analyzed in each strain. (B) A small region in the PxylX region is shown, with the XylR binding site underlined. Sequences above and below the line show the different mutations detected.

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Table 1
Bacterial strains and plasmids used in this study.

Strain	Relevant Genotype	Source
C. crescentus
NA1000	Parental strain, C. crescentus CB15 derivative	Evinger and Agabian, 1977
CS606	NA1000 ΔblaA	*West et al.,* 2002**West L, Yang D and Stephens C (2002) Use of the Caulobacter crescentus genome sequence to develop a method for systematic genetic mapping. J Bacteriol 184:2155–2166.
GM40	NA1000 imuC::Spec^R	*Galhardo et al.,* 2005**Galhardo RS, Rocha RP, Marques MV and Menck CFM (2005) An SOS-regulated operon involved in damage-inducible mutagenesis in Caulobacter crescentus. Nucleic Acids Res 33:2603–2614.
GM50	NA1000 dinB::Spec^R	*Galhardo et al.,* 2005**Galhardo RS, Rocha RP, Marques MV and Menck CFM (2005) An SOS-regulated operon involved in damage-inducible mutagenesis in Caulobacter crescentus. Nucleic Acids Res 33:2603–2614.
RSG113	NA1000 ΔblaA ΔxylX::blaA	This study
RSG124	NA1000 ΔblaA ΔxylX::blaA dinB::Spec^R	This study
RSG247	NA1000 ΔblaA ΔxylX::blaA imuC::Spec^R	This study
RSG317	NA1000 cI (Ind^-) λpR tetA	This study
RSG318	NA1000 cI (Ind^-) λpR tetA imuC::Spec^R	This study
RSG319	NA1000 cI (Ind^-) λpR tetA dinB::Spec^R	This study
E. coli
MG1655, cI marker	MG1655 attλ:cI (Ind^-) λpR tetA Δara:FRT ΔmetRE:FRT	*Bjedov et al.,* 2007**Bjedov I, Dasgupta CN, Slade D, Le Blastier S, Selva M and Matic I (2007) Involvement of Escherichia coli DNA polymerase IV in tolerance of cytotoxic alkylating DNA lesions in vivo. Genetics 176:1431–1440.)
Plasmids
pNPTS138	pNPTS129 derivative, oriT sacB Kan^R	Tsai and Alley, 2001
pNPTxylblaE2	In frame substitution of xylX by blaA with flanking regions, cloned in pNPTS138	This study
pMCS7	Cloning vector, non-replicating in C. crescentus	Thanbichler et al., 2007
pMCSCI	pMCS7 containing the cItet cassette and ~500 bp of DNA for homologous recombination in the C. crescentus chromosome	This study

[1] Send correspondence to Rodrigo S. Galhardo. Universidade de São Paulo, Instituto de Ciências Biomédicas, Departamento de Microbiologia, Butantã, São Paulo, SP, Brazil. E-mail: rgalhard@usp.br.

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Role of error-prone DNA polymerases in spontaneous mutagenesis in Caulobacter crescentus

Abstract