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W tym Artykule

  • Podsumowanie
  • Streszczenie
  • Protokół
  • Wyniki
  • Dyskusje
  • Ujawnienia
  • Podziękowania
  • Materiały
  • Odniesienia
  • Przedruki i uprawnienia

Podsumowanie

An efficient genome-wide single gene mutation method has been established using Streptococcus sanguinis as a model organism. This method has achieved via high throughput recombinant PCRs and transformations.

Streszczenie

Transposon mutagenesis and single-gene deletion are two methods applied in genome-wide gene knockout in bacteria 1,2. Although transposon mutagenesis is less time consuming, less costly, and does not require completed genome information, there are two weaknesses in this method: (1) the possibility of a disparate mutants in the mixed mutant library that counter-selects mutants with decreased competition; and (2) the possibility of partial gene inactivation whereby genes do not entirely lose their function following the insertion of a transposon. Single-gene deletion analysis may compensate for the drawbacks associated with transposon mutagenesis. To improve the efficiency of genome-wide single gene deletion, we attempt to establish a high-throughput technique for genome-wide single gene deletion using Streptococcus sanguinis as a model organism. Each gene deletion construct in S. sanguinis genome is designed to comprise 1-kb upstream of the targeted gene, the aphA-3 gene, encoding kanamycin resistance protein, and 1-kb downstream of the targeted gene. Three sets of primers F1/R1, F2/R2, and F3/R3, respectively, are designed and synthesized in a 96-well plate format for PCR-amplifications of those three components of each deletion construct. Primers R1 and F3 contain 25-bp sequences that are complementary to regions of the aphA-3 gene at their 5' end. A large scale PCR amplification of the aphA-3 gene is performed once for creating all single-gene deletion constructs. The promoter of aphA-3 gene is initially excluded to minimize the potential polar effect of kanamycin cassette. To create the gene deletion constructs, high-throughput PCR amplification and purification are performed in a 96-well plate format. A linear recombinant PCR amplicon for each gene deletion will be made up through four PCR reactions using high-fidelity DNA polymerase. The initial exponential growth phase of S. sanguinis cultured in Todd Hewitt broth supplemented with 2.5% inactivated horse serum is used to increase competence for the transformation of PCR-recombinant constructs. Under this condition, up to 20% of S. sanguinis cells can be transformed using ~50 ng of DNA. Based on this approach, 2,048 mutants with single-gene deletion were ultimately obtained from the 2,270 genes in S. sanguinis excluding four gene ORFs contained entirely within other ORFs in S. sanguinis SK36 and 218 potential essential genes. The technique on creating gene deletion constructs is high throughput and could be easy to use in genome-wide single gene deletions for any transformable bacteria.

Protokół

1. Primer Design

  1. Primers are designed using in house scripts based on the S. sanguinis SK36 genome sequence. Three sets of primers, F1/R1, F2/R2, and F3/R3 are designed for amplification of the 1-kb upstream sequence of the target gene, the aphA-3 gene encoding kanamycin resistance (Kmr) protein3 and the 1-kb downstream sequence of the target gene, respectively (Figure 1). Among these primers, F1 and R3 are designed using ePrimer3 in the EMBOSS suite of programs (http://emboss.sourceforge.net/apps/cvs/emboss/apps/index.html) to amplify flanking regions upstream or downstream of the target gene. Gene specific primers, R1 and F3, are designed based upon the 5' and 3' sequences of the target gene. R1 and F3 primers contain 25-bp adaptor sequences at their 5' end that are complementary to the aphA-3 gene. The melting temperatures of each primer were designed to be as close as possible to 60 °C to enable use of a uniform annealing temperature for all PCR reactions in 96-well format.
  2. F1, R1, F3 and R3 primers are synthesized in 96-well plates based on a gene order. Each plate contains one type of primers in the same gene order. Dilute the primers in 96-well working primer plate to a final concentration of 10 μM for PCR amplification using a multichannel pipette.

2. High-throughput PCR Amplification and Purification

  1. To high-throughput amplify 1-kb upstream or downstream of the target S. sanguinis genes, assemble a PCR cocktail mixture on ice in a 15-ml conical tube containing 1640 μl ddH2O, 250 μl 10xHigh Fidelity PCR Buffer, 200 μl of 10 mM dNTP mixture, 100 μl of 50 mM MgSO4, 100 μl of 10 ng/ μl S. sanguinis SK36 genomic DNA and 10 μl Platinum Taq DNA polymerase high fidelity and transfer 23 μl of the mixture into each well on 96-well PCR plate using a multichannel pipette. Transfer 1 μl of each F1 and R1 (or F3 and R3) from the 10 μM working primer plates to the PCR plate using multichannel pipette. Seal the PCR plate and perform amplification at 94 °C for 1 min, and 30 cycles of 94 °C for 30 sec, 54 °C for 30 sec and 68 °C for 1.5 min.
  2. Prepare 1% agarose gel containing ethidium bromide with 48 wells fitting multichannel pipette loading. Mix 4 μl PCR product with 1 μl of 5xDNA loading buffer on 96-well plate and load the samples on agarose gel using a 10-μl multichannel pipette. Run electrophoresis at 135 V for 30 min. Examine the band on gel under UVP documentation and analysis system.
  3. Purify the PCR products by PureLink 96 PCR purification kit using centrifugation according to the manufacturer's instruction. For eluting DNA, add 40 μl sterile ddH2O to the well of the binding plate.
  4. Randomly pick several purified amplicons on the plate to examine the DNA concentrations using NanoDrop spectrophotometer. Adjust the concentration of amplicons on plate to ~10 ng/μl.
  5. A plasmid containing Kmr cassette is digested using EcoRI as PCR template. The digested plasmid is purified by QIAquick PCR purification kit and the linear plasmid DNA is adjusted to final DNA concentration 10 ng/μl. Assemble 25 μl mixture for Kmr cassette amplicon including 16.4 μl ddH2O, 2.5 μl 10xHigh Fidelity PCR Buffer, 2 μl of 10 mM dNTP mixture, 1 μl of 50 mM Mg SO4, 1 μl of 10 μM F2, 1 μl of 10 μM R2, 1 μl linear plasmid DNA and 0.1 μl Platinum Taq DNA polymerase high fidelity. Perform PCR amplification at 94 °C for 1 min, and 30 cycles of 94 °C for 30 sec, 55 °C for 30 sec and 68 °C for 1 min. Examine the PCR product by gel electrophoresis on 1% agarose. Pool a bulk of the Kmr cassette amplicon from 10 individual PCR purified by QIAquick PCR purification kit. Adjust the amplicon concentration to 10 ng/μl.
  6. To obtain the final linear recombinant PCR amplicon, three PCR amplicons are combined with each 1 μl (in nearly equal-molar amounts) in one PCR plate well as the PCR template. Other PCR components is added including 14.4 μl ddH2O, 2.5 μl 10xHigh Fidelity PCR Buffer, 2 μl of 10 mM dNTP mixture, 1 μl of 50 mM Mg SO4, 1 μl of 10 μM F1, 1 μl of 10 μM R3, 0.1 μl Platinum Taq DNA polymerase high fidelity. PCR amplification is performed at 94 °C for 2 min, 30 cycles of 94 °C for 30 sec 55 °C for 30 sec and 68 °C for 3.5 min, and finally 68 °C for 4 min.
  7. Examine the PCR amplicons on agarose gel. Purify and quantify the PCR amplicons as described above. Freeze the recombined PCR amplicons at -20 °C.

3. Competent Cells Preparation

  1. Todd Hewitt broth is prepared, adjusted pH to 7.6 using 10 N NaOH, heated to boil and then cooled to room temperature and sterilized using 0.22 μm polystyrene filter4. Add 300 μl heat-inactivated horse sera (final concentration to 2.5%) to 11.7 ml Todd Hewitt broth in 15-ml conical tube to make up TH+HS medium. Aliquot TH+HS medium into 2 ml and 10 ml in tubes.
  2. Inoculate 5 μl of stock S. sanguinis SK36 frozen at -80 °C into 2 ml TH+HS medium and incubate the culture overnight with capping tightly at 37 °C, accompanied by pre-incubating the 10 ml-TH+HS tube.
  3. After overnight, transfer 50 μl culture into 10 ml TH+HS and incubate the tube at 37 °C for 3 hr (corresponding to OD660 of 0.07-0.08), immediately using for transformation.

4. Cell Transformation and Antibiotic Selection

  1. Add 2 μl of 70 ng S. sanguinis SK36 competence stimulating peptide (CSP) and 2 μl linear recombinant PCR amplicon (~50 ng) to Eppendorf tubes on 96-well block and pre-warm them at 37 °C. Transfer 330 μl of 3 hr-incubated SK36 culture into each tube. Incubate at 37 °C for 1 hr. Replace DNA with sterile ddH2O as control.
  2. Place the block on ice and spread 100 μl of each transformation on brain heart infusion (BHI) agar plate with 500 μg/ml kanamycin. Incubate the plates at 37 °C for 2 d under microaerobic conditions.

5. Mutant Confirmation and Storage

  1. For each replacement mutant, randomly pick up 2 individual colonies, inoculate the colony into 5 ml BHI containing 500 μg/ml kanamycin and incubate the inoculum microaerobically overnight at 37 °C. Cryopreserve each culture in 30% glycerol at -80 °C
  2. To examine whether the mutant containing the expected gene replacement, perform colony PCR for each mutant using F1 and R3 primers in 96-well PCR plate. About 1-μl overnight culture from individual colony is used as the DNA template in 25-μl PCR-amplification reaction. PCR is performed at 94 °C for 5 min, 35 cycles of 94 °C for 30 sec, 55 °C for 30 sec and 68 °C for 3.5 min, and finally 68 °C for 4 min.
  3. To precisely identify double-band mutants or contaminant PCR amplicon, examine the PCR amplicon by electrophoresis for 4 hr on >12 cm long 2% agarose gel with ethidium bromide staining. Under this agarose gel electrophoresis condition, any amplicons with ≥ 100 bp difference were clearly identified. When bands resulting from amplification of the Kmr cassette and the wild-type gene are anticipated to differ by < 100 bp, an internal T1 primer is used to determine whether a wild-type gene can be detected by PCR.
  4. To further confirm the deletion, the amplicons are purified by PureLink 96 PCR purification kit and sequenced using the P1 primer which binds to the Kmr cassette. Keep only correct mutants confirmed by sequencing.

Wyniki

After PCR amplification using primers F1 and R1, and F3 and R3, approximately 1-kb upstream and downstream of each S. sanguinis gene were obtained in 96-well format, respectively (Figure 2A). Under our PCR conditions and using designed primers, a specific product was amplified from S. sanguinis genomic DNA in each PCR reaction. This result indicated the primers were highly specific to the targets of S. sanguinis. Through PCR re-amplification using primers F1 and R3 and t...

Dyskusje

To minimize the possible polar effects of the replacement of one targeted gene with exogenous antibiotics gene on neighboring genes, two steps are taken while initial primer designing. For most of deleted genes, the primers R1 and F3 are designed to delete the coding region from 6 bp following the start codon to 30 bp prior to the stop codon. The last 30 base pairs are retained to protect potential ribosomal binding site used by the adjacent downstream gene. The retained region between two neighboring genes is extended t...

Ujawnienia

No conflicts of interest declared.

Podziękowania

This work was supported by grants R01DE018138 from the National Institutes of Health (PX) and in part, by Virginia Commonwealth University Presidential Research Incentive Program (PRIP) 144602-3 (PX). We thank Drs. Lei Chen, Yuetan Dou and Xiaojing Wang for assisting with the construction of genome wide mutants. We also thank the DNA Core Facility at Virginia Commonwealth University for DNA sequencing.

Materiały

NameCompanyCatalog NumberComments
Primer F2Integrated DNA TechnologiesTGACTAACTAGGAGGAATAAATG
GCTAAAATGAGAATAT
Primer R2ibidCATTATTCCCTCCAGGTACTAAAA
CAATTCATCCAGT
Primer F2pibidGATAAACCCAGCGAACCATTTGA
Primer P1ibidGCTTATATACCTTAGCAGGAGACA
Primer P2ibidGTATGACATTGCCTTCTGCGTCC
Primer 5' end_R1_seqibidGCCATTTATTCCTCCTAGTTAGTCA
Primer 5' end_F3_seqibidGTTTTAGTACCTGGAGGGAATAATG
Primer 5' end_R1p_seqibidCCTCAAATGGTTCGCTGGGTTTATC
CSPSynprepSequence:NH2-DLRGVPNPWGWIFGR-COOH
DNA Polymerase Invitrogen11304-102Platinum Taq DNA Polymerase High Fidelity
EcoRINew England Biolabs IncR0101SRestriction enzyme
AgarAmerican BioanalyticalAB01185
AgarosePromegaV3125
BHIBD Biosciences237500Brain Heart Infusion
Horse serumFisher ScientificSH3007403Horse serum
KmFisher ScientificBP906-5Kanamycin
TH brothBD Biosciences249240Todd Hewitt broth
PureLink 96InvitrogenK310096PureLink 96 PCR purification kit
QIAquickQiagen28106QIAquick PCR purification kit
FilterCorning4311170.22 μm polystyrene filter
Anoxomat SystemMart Microbiology b.v.Anoxomat Mark II
Benchtop centrifugeThermo Scientific75004377Sorvall Legend RT Plus microplate rotor
Gel DocumentationUVP LLCBioDoc-It 210
IncubatorFisher Scientific11-690-625DIsotemp
Labnet's Gel XLLabnetE0160Labnet's Gel XL
MicrocentrifugeEppendorf22621408Microcentrifuge 5415 R
Multichannel pipettesThermo Scientfic4661040, 4661020Finnpipette F1
Thermal CyclerApplied Biosystems Inc.N805-0200GeneAmp PCR system 9700

Odniesienia

  1. Sassetti, C. M., Boyd, D. H., Rubin, E. J. Genes required for mycobacterial growth defined by high density mutagenesis. Mol. Microbiol. 48, 77-84 (2003).
  2. Kobayashi, K., et al. Essential Bacillus subtilis genes. Proc. Natl. Acad. Sci. U.S.A. 100, 4678-4683 (2003).
  3. Trieu-Cuot, P., Courvalin, P. Nucleotide sequence of the Streptococcus faecalis plasmid gene encoding the 3'5"-aminoglycoside phosphotransferase type III. Gene. 23, 331-341 (1983).
  4. Paik, S., et al. Identification of virulence determinants for endocarditis in Streptococcus sanguinis by signature-tagged mutagenesis. Infect. Immun. 73, 6064-6074 (2005).
  5. Lukomski, S., et al. Nonpolar inactivation of the hypervariable streptococcal inhibitor of complement gene (sic) in serotype M1 Streptococcus pyogenes significantly decreases mouse mucosal colonization. Infect. Immun. 68, 535-542 (2000).
  6. Baba, T., et al. Construction of Escherichia coli K-12 in-frame, single-gene knockout mutants: the Keio collection. Mol. Syst. Biol. 2, (2006).
  7. de Berardinis, V. A complete collection of single-gene deletion mutants of Acinetobacter baylyi ADP1. Mol. Syst. Biol. 4, 174 (2008).
  8. Rodriguez, A. M., et al. Physiological and molecular characterization of genetic competence in Streptococcus sanguinis. Mol. Oral. Microbiol. 26, 99-116 (2011).
  9. Perry, D., Kuramitsu, H. K. Genetic transformation of Streptococcus mutans Infect. Immun. 32, 1295-1297 (1981).
  10. Pakula, R., Walczak, W. On the nature of competence of transformable streptococci. J. Gen. Microbiol. 31, 125-133 (1963).
  11. Datsenko, K. A., Wanner, B. L. One-step inactivation of chromosomal genes in Escherichia coli K-12 using PCR products. Proc. Natl. Acad. Sci. U.S.A. 97, 6640-6645 (2000).
  12. Xu, P., et al. Genome-wide essential gene identification in Streptococcus sanguinis. Sci. Rep. 1, (2011).

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Genome wide Gene DeletionsStreptococcus SanguinisHigh Throughput PCRTransposon MutagenesisSingle gene DeletionBacteriaGene KnockoutMutant LibraryPartial Gene InactivationHigh throughput TechniqueModel OrganismGene Deletion ConstructKanamycin Resistance ProteinPrimersPCR Amplification

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