Enhanced method for microbial community DNA extraction and purification from agricultural yellow loess soil

Kathiravan, Mathur Nadarajan; Gim, Geun Ho; Ryu, Jaewon; Kim, Pyung Il; Lee, Chul Won; Kim, Si Wouk

doi:10.1007/s12275-015-5454-0

Cited by 9 publications

(8 citation statements)

References 29 publications

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“…To compensate for the low DNA extraction efficiency of lysozyme for most Gram-negative bacteria, a treatment step with proper ultrasonic disruption was used in the CLU method, which could break down the cell walls of Gram-negative bacteria and allowed good liberation of the DNA. In addition, the incubation temperature during the process of lysozyme lysis was usually maintained at 37 °C in previous studies (Kathiravan et al 2015 ; Bag et al 2016 ). However, some investigators noted that the activity of lysozyme from egg whites increased gradually with increasing temperature within the range of 25–65 °C (Liu et al 2008 ).…”

Section: Discussionmentioning

confidence: 99%

“…In early studies, conventional culture-dependent techniques were used; however, only a small percentage of the bacterial flora was identified (Kathiravan et al 2015 ). Recently, molecular techniques, including but not limited to denatured gradient gel electrophoresis (Li et al 2011 ), fluorescence in situ hybridization (Hoffmann et al 2006 ) and 16S rDNA high-throughput sequencing (Gajardo et al 2016 ), have been used successfully to analyze the complex microbial community from fish intestines.…”

Section: Introductionmentioning

confidence: 99%

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A modified method for genomic DNA extraction from the fish intestinal microflora

Han

Sun

et al. 2018

AMB Expr

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A modified genomic DNA extraction method named the combination of lysozyme and ultrasonic lysis (CLU) method was used to analyze the fish intestinal microflora. In this method, the physical disruption and chemical lysis steps were combined, and some parameters in the key steps were adjusted. In addition, the results obtained by this method were compared with the results obtained by the Zirmil-beating cell disruption method and the QIAamp Fast DNA Stool Mini Kit. The OD260/OD280 ratio and concentration of the DNA extracted using the CLU method were 2.02 and 282.8 µg/µL, respectively; when the incubation temperatures for lysozyme and RNase were adjusted to 37 °C, those values were 2.08 and 309.8 µg/µL, respectively. On the agarose gel, a major high-intensity, discrete band of more than 10 kb was found for the CLU method. However, the smearing intensity of degraded DNA was lower when the incubation temperatures were 60 °C for lysozyme and 30 °C for RNase than when incubation temperatures of 37 °C for lysozyme and 37 °C for RNase were used. The V3 variable region of the prokaryotic 16S rDNA was amplified, and an approximately 600-bp fragment was observed when the DNA extracted using the CLU method was used as a template. The CLU method is simple and cost effective, and it yields high-quality, unsheared, high-molecular-weight DNA, which is comparable to that obtained with a commercially available kit. The extracted DNA has potential for applications in critical molecular biology techniques.

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

A modified method for genomic DNA extraction from the fish intestinal microflora

Han

Sun

et al. 2018

AMB Expr

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“…Over the last decade, an increasing number of studies have focused on the gut microbiota of fish (Narrowe et al., ; Xia et al., ). In early studies, conventional culture‐dependent techniques were used; however, only a small percentage of the resulting bacterial flora was identified (Kathiravan et al., ). Recently, new technologies based on meta‐genomics/high‐throughput sequencing have been developed and successfully applied to analyzing the complex bacterial ecosystem of the gut.…”

Section: Introductionmentioning

confidence: 99%

Biases from different DNA extraction methods in intestine microbiome research based on 16S rDNA sequencing: a case in the koi carp, Cyprinus carpio var. Koi

Han

Sun

et al. 2018

MicrobiologyOpen

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This study examined the technical bias associated with different DNA extraction methods used in microbiome research. Three methods were used to extract genomic DNA from the same intestinal microbiota sample that was taken from the koi carp Cyprinus carpio var. koi, after which their microbial diversity and community structure were investigated on the basis of a 16S rDNA high-throughput sequencing analysis. Biased results were observed in relation to the number of reads, alpha diversity indexes and taxonomic composition among the three DNA extraction protocols. A total of 1,381 OTUs from the intestinal bacteria were obtained, with 852, 759, and 698 OTUs acquired, using the Lysozyme and Ultrasonic Lysis method, Zirmil-beating Cell Disruption method, and a QIAamp Fast DNA Stool Mini Kit, respectively. Additionally, 336 OTUs were commonly acquired, using the three methods. The results showed that the alpha diversity indexes (Rarefaction, Shannon, and Chao1) of the community that were determined using the Lysozyme and Ultrasonic Lysis method were higher than those obtained with the Zirmil-beating Cell Disruption method, while the Zirmil method results were higher than those measured, using the QIAamp Fast DNA Stool Mini Kit. Moreover, all the major phyla (ratio>1%) could be identified with all three DNA extraction methods, but the phyla present at a lower abundance (ratio <1%) could not. Similar findings were observed at the genus level. Taken together, these findings indicated that the bias observed in the results about the community structure occurred primarily in OTUs with a lower abundance. The results of this study demonstrate that possible bias exists in community analyses, and researchers should therefore be conservative when drawing conclusions about community structures based on the currently available DNA extraction methods.

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“… 5 Accordingly, the isolation of high-quality DNA that covers the whole microbial diversity in the original sample was phrased as a limiting step for the construction of metagenomic libraries and other DNA based metagenomic projects. 6 …”

Section: Introductionmentioning

confidence: 99%

“…In these regards, many studies have reported the development of methods and even commercial kits for mDNA extraction. 5 , 6 However, still, there is a surge in developing, improving, and optimizing new or current protocols for mDNA extraction from different types of samples. A metagenomic DNA extraction must be followed by a quality control of the extracted DNA.…”

Section: Introductionmentioning

confidence: 99%

Illumina sequencing and assessment of new cost-efficient protocol for metagenomic-DNA extraction from environmental water samples

Hassan

Essam

Megahed

2018

Brazilian Journal of Microbiology

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In this study, the development and assessment of a modified, efficient, and cost-efficient protocol for mDNA (metagenomic DNA) extraction from contaminated water samples was attempted. The efficiency of the developed protocol was investigated in comparison to a well-established commercial kit (Epicentre, Metagenomic DNA Isolation Kit for Water). The comparison was in terms of degree of shearing, yield, purity, duration, suitability for polymerase chain reaction and next-generation sequencing in addition to the quality of next-generation sequencing data. The DNA yield obtained from the developed protocol was 2.6 folds higher than that of the commercial kit. No significant difference in the alpha (Observed species, Chao1, Simpson and PD whole tree) and beta diversity was found between the DNA samples extracted by the commercial kit and the developed protocol. The number of high-quality sequences of the samples extracted by the developed method was 20% higher than those obtained by the samples processed by the kit. The developed economic protocol successfully yielded high-quality pure mDNA compatible with complex molecular applications. Thus we propose the developed protocol as a gold standard for future metagenomic studies investigating a large number of samples.

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Enhanced method for microbial community DNA extraction and purification from agricultural yellow loess soil

Cited by 9 publications

References 29 publications

A modified method for genomic DNA extraction from the fish intestinal microflora

A modified method for genomic DNA extraction from the fish intestinal microflora

Biases from different DNA extraction methods in intestine microbiome research based on 16S rDNA sequencing: a case in the koi carp, Cyprinus carpio var. Koi

Illumina sequencing and assessment of new cost-efficient protocol for metagenomic-DNA extraction from environmental water samples

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