Gene/Protein Disease Symptom Drug Enzyme Compound
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Query: EC:3.1.21.1 (DNase)
 7,655 document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)

Schizophyllan is a beta-(1-->3)-D-glucan and can form a novel complex with some single-chains of DNAs. As the preceding paper revealed, the polynucleotide bound in the complex is more stable to nuclease-mediated hydrolysis than the polynucleotide itself (i.e., naked polynucleotide). This paper examined possibility to apply this complex to an antisense DNA carrier, using an in vitro (cell-free) transcription/translation assay. In this assay, we used a plasmid DNA coding a green fluorescence protein (GFP) and an antisense DNA designed to hybridize the ribosome-binding site in the GFP-coded mRNA. When the antisense DNA was administered as the complex, a lower GFP expression efficiency (or higher antisense effect) is observed over naked DNA. This is because the antisense DNA in the complex is protected from the attack of deoxyribonuclease. When exonuclease I, which specifically hydrolyzes single DNA chains, was present in the GEP assay system, the antisense effect was not changed for the complex while being weakened in the naked antisense DNA system. These results imply that the exonuclease I cannot hydrolyze the antisense DNA in the complex, while it can hydrolyze naked DNA to reduce its antisense effect.
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PMID:Antisense oligonucleotides bound in the polysaccharide complex and the enhanced antisense effect due to the low hydrolysis. 1496 45

To assess the contributions of single-strand DNases (ssDNases) to recombination in a recBCD+ background, we studied 31 strains with all combinations of null alleles of exonuclease I (delta xon), exonuclease VII (xseA), RecJ DNase (recJ), and SbcCD DNase (sbcCD) and exonuclease I mutant alleles xonA2 and sbcB15. The xse recJ sbcCD delta xon and xse recJ sbcCD sbcB15 quadruple mutants were cold sensitive, while the quadruple mutant with xonA2 was not. UV sensitivity increased with ssDNase deficiencies. Most triple and quadruple mutants were highly sensitive. The absence of ssDNases hardly affected P1 transductional recombinant formation, and conjugational recombinant production was decreased (as much as 94%) in several cases. Strains with sbcB15 were generally like the wild type. We determined that the sbcB15 mutation caused an A183V exchange in exonuclease motif III and identified xonA2 as a stop codon eliminating the terminal 8 amino acids. Purified enzymes had 1.6% (SbcB15) and 0.9% (XonA2) of the specific activity of wild-type Xon (Xon+), respectively, with altered activity profiles. In gel shift assays, SbcB15 associated relatively stably with 3' DNA overhangs, giving protection against Xon+. In addition to their postsynaptic roles in the RecBCD pathway, exonuclease I and RecJ are proposed to have presynaptic roles of DNA end blunting. Blunting may be specifically required during conjugation to make DNAs with overhangs RecBCD targets for initiation of recombination. Evidence is provided that SbcB15 protein, known to activate the RecF pathway in recBC strains, contributes independently of RecF to recombination in recBCD+ cells. DNA end binding by SbcB15 can also explain other specific phenotypes of strains with sbcB15.
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PMID:Effects of single-strand DNases ExoI, RecJ, ExoVII, and SbcCD on homologous recombination of recBCD+ strains of Escherichia coli and roles of SbcB15 and XonA2 ExoI mutant enzymes. 1796 70

Prevailing conventional microbial detection methods depend largely on microbial cultivation in selective media that requires several days. Polymerase chain reaction (PCR)-based methods, including quantitative reverse transcription PCR, are also rapid and useful methods for identification of target microbes, although for practical use they still suffer from disadvantages such as contamination problems and cost. Here we demonstrate that RNA-primed rolling circle amplification (RPRCA) using phi29 DNA polymerase, a precircularized probe, and SYBR Green II achieved real-time detection of specific messenger RNA (mRNA) from living microbes. The precircularized DNA probe was prepared by intramolecular ligation using CircLigase and treated by exonuclease I to eliminate uncircularized oligonucleotide, thereby significantly reducing potential noise by nonspecific amplified DNA by-products that affect successive RPRCA. When in vitro transcribed green fluorescent protein (GFP) mRNA was used as a primer, RPRCA could specifically detect at least 1 fmol of this mRNA in the presence of a precircularized probe that had a sequence complementary to the 3' terminus of mRNA without reverse transcription. This method could also detect expressed GFP mRNA present in 10 ng of total RNA isolated from Escherichia coli without DNase treatment. These data suggest that RPRCA has the potential to be a direct, rapid, and convenient method for detecting microbial mRNA.
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PMID:Direct detection of green fluorescent protein messenger RNA expressed in Escherichia coli by rolling circle amplification. 2023 Jul 71


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