2006
DOI: 10.1271/bbb.70.340
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Isolation and Characterization of a Bluegill-Degrading Microorganism, and Analysis of the Root Hair-Promoting Effect of the Degraded Products

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Cited by 7 publications
(2 citation statements)
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“…The DNA extraction method for 16S rDNA sequencing and sequence data analysis were described previously (Sanpa et al 2006). The 16S rDNA of the isolates was amplified by polymerase chain reaction (PCR) with primers 20F (5 0 -TGTAA TCGTC GGCCA GTAGA GTTTG ATCCT GGCTC -3 0 ) and 1510R (5 0 -CAGGA AACAG CTATG ACCGG CTACC TTGTT ACGAC T-3 0 ).…”
Section: Methodsmentioning
confidence: 99%
“…The DNA extraction method for 16S rDNA sequencing and sequence data analysis were described previously (Sanpa et al 2006). The 16S rDNA of the isolates was amplified by polymerase chain reaction (PCR) with primers 20F (5 0 -TGTAA TCGTC GGCCA GTAGA GTTTG ATCCT GGCTC -3 0 ) and 1510R (5 0 -CAGGA AACAG CTATG ACCGG CTACC TTGTT ACGAC T-3 0 ).…”
Section: Methodsmentioning
confidence: 99%
“…Cultures of the selected strains were analyzed for the WSP content, and those showing a higher amount (1,000 mg ml 1 ) were selected for taxonomic classification. For taxonomic classification, 16S rRNA gene sequences were analyzed following the procedures of Koma et al (2003) and Sanpa et al (2006). The 16S rRNA gene primers 20F (5 -TGTAATCGTCGGCCAG TAGAGTTTGATCCTGGCTC-3 ) and 1510R (5 -CAG were used for PCR to amplify the 16S rRNA gene.…”
Section: Methodsmentioning
confidence: 99%