Development of a versatile cassette for directional genome walking using cassette ligation-mediated PCR and its application in the cloning of complete lipolytic genes from Bacillus species

Since the invention of the PCR technology, adaptation techniques to clone DNA fragments flanking the known sequence continue to be developed. We describe a perfectly annealed cassette available in almost unlimited quantities with variable sticky–and blunt–end restriction enzyme recognition sites for...

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Published inJournal of microbiological methods Vol. 61; no. 2; pp. 225 - 234
Main Authors Nthangeni, Mulalo B., Ramagoma, Faranani, Tlou, Matsobane G., Litthauer, Derek
Format Journal Article
LanguageEnglish
Published Shannon Elsevier B.V 01.05.2005
Elsevier Science
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Abstract Since the invention of the PCR technology, adaptation techniques to clone DNA fragments flanking the known sequence continue to be developed. We describe a perfectly annealed cassette available in almost unlimited quantities with variable sticky–and blunt–end restriction enzyme recognition sites for efficient restriction and ligation with the restricted target genomic DNA. The cassette provides a 200-bp sequence, which is used to design a variety of cassette-specific primers. The dephosphorylation prevents cassette self-ligation and creates a nick at the cassette: target genome DNA ligation site suppressing unspecific PCR amplifications. We introduce the single-strand amplification PCR (SSA-PCR) technique where a lone known locus-specific primer is firstly used to enrich the targeted template DNA strand resulting in significant PCR product specificity during the second round conventional nested PCR. The distance between the known locus-specific primer and the nearest location of the restriction enzyme used determined the length of the obtained PCR product. We used this technique to walk downstream into the isochorismatase and upstream into the hypothetical conserved genes flanking the mature extracellular lipase gene from Bacillus licheniformis. We further demonstrated the potential of the technique as a cost-effective method during PCR-based prospecting for novel genes by designing “universal” degenerate primers that detected homologues of Family VII bacterial lipolytic genes in Bacillus species. The cassette ligation-mediated PCR was used to clone complete nucleotide sequences encoding functional lipolytic genes from B. licheniformis and Bacillus pumilus.
AbstractList Since the invention of the PCR technology, adaptation techniques to clone DNA fragments flanking the known sequence continue to be developed. We describe a perfectly annealed cassette available in almost unlimited quantities with variable sticky-and blunt-end restriction enzyme recognition sites for efficient restriction and ligation with the restricted target genomic DNA. The cassette provides a 200-bp sequence, which is used to design a variety of cassette-specific primers. The dephosphorylation prevents cassette self-ligation and creates a nick at the cassette: target genome DNA ligation site suppressing unspecific PCR amplifications. We introduce the single-strand amplification PCR (SSA-PCR) technique where a lone known locus-specific primer is firstly used to enrich the targeted template DNA strand resulting in significant PCR product specificity during the second round conventional nested PCR. The distance between the known locus-specific primer and the nearest location of the restriction enzyme used determined the length of the obtained PCR product. We used this technique to walk downstream into the isochorismatase and upstream into the hypothetical conserved genes flanking the mature extracellular lipase gene from Bacillus licheniformis. We further demonstrated the potential of the technique as a cost-effective method during PCR-based prospecting for novel genes by designing ''universal'' degenerate primers that detected homologues of Family VII bacterial lipolytic genes in Bacillus species. The cassette ligation-mediated PCR was used to clone complete nucleotide sequences encoding functional lipolytic genes from B. licheniformis and Bacillus pumilus.
Since the invention of the PCR technology, adaptation techniques to clone DNA fragments flanking the known sequence continue to be developed. We describe a perfectly annealed cassette available in almost unlimited quantities with variable sticky–and blunt–end restriction enzyme recognition sites for efficient restriction and ligation with the restricted target genomic DNA. The cassette provides a 200-bp sequence, which is used to design a variety of cassette-specific primers. The dephosphorylation prevents cassette self-ligation and creates a nick at the cassette: target genome DNA ligation site suppressing unspecific PCR amplifications. We introduce the single-strand amplification PCR (SSA-PCR) technique where a lone known locus-specific primer is firstly used to enrich the targeted template DNA strand resulting in significant PCR product specificity during the second round conventional nested PCR. The distance between the known locus-specific primer and the nearest location of the restriction enzyme used determined the length of the obtained PCR product. We used this technique to walk downstream into the isochorismatase and upstream into the hypothetical conserved genes flanking the mature extracellular lipase gene from Bacillus licheniformis. We further demonstrated the potential of the technique as a cost-effective method during PCR-based prospecting for novel genes by designing “universal” degenerate primers that detected homologues of Family VII bacterial lipolytic genes in Bacillus species. The cassette ligation-mediated PCR was used to clone complete nucleotide sequences encoding functional lipolytic genes from B. licheniformis and Bacillus pumilus.
Author Litthauer, Derek
Nthangeni, Mulalo B.
Tlou, Matsobane G.
Ramagoma, Faranani
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Issue 2
Keywords T m
CSP
SSA-PCR
ORF
LSP
Single-strand amplification PCR
Cassette ligation-mediated PCR
Family VII lipolytic genes
PCR
bp
Nucleotide sequence
Bacillus licheniformis
Enzyme
Genomics
Transposable element
Flanking sequence
Bacillaceae
IS element
Polymerase chain reaction
Bacillales
Gene
DNA
Bacillus pumilus
Development
Bacteria
Genome
Recognition
Adaptation
Language English
License CC BY 4.0
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Snippet Since the invention of the PCR technology, adaptation techniques to clone DNA fragments flanking the known sequence continue to be developed. We describe a...
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SubjectTerms Amino Acid Sequence
Bacillus
Bacillus - enzymology
Bacillus - genetics
Bacillus licheniformis
Bacillus pumilus
Bacteriology
Bacteriophage lambda - genetics
Base Sequence
Biological and medical sciences
Carboxylesterase - genetics
Carboxylesterase - metabolism
Cassette ligation-mediated PCR
Cloning, Molecular
DNA, Bacterial - genetics
Family VII lipolytic genes
Fundamental and applied biological sciences. Psychology
Genome, Bacterial
Lipase - genetics
Lipase - metabolism
Microbiology
Miscellaneous
Molecular Sequence Data
Polymerase Chain Reaction - methods
Sequence Alignment
Single-strand amplification PCR
Title Development of a versatile cassette for directional genome walking using cassette ligation-mediated PCR and its application in the cloning of complete lipolytic genes from Bacillus species
URI https://dx.doi.org/10.1016/j.mimet.2004.11.021
https://www.ncbi.nlm.nih.gov/pubmed/15722149
https://search.proquest.com/docview/17562423
https://search.proquest.com/docview/20030528
https://search.proquest.com/docview/67442941
Volume 61
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