Your search keyword '"dna extraction"' showing total 287 results

1. Extraction of high-quality metagenomic DNA from the lichens Flavoparmelia caperata and Peltigera membranacea.

Author

Gregoris, Kalea and Pope, Welkin H.

Subjects

*SODIUM dodecyl sulfate, *NUCLEIC acid isolation methods, *INDUSTRIAL pollution, *NUCLEIC acids, *TEMPERATE forests

Abstract

Lichens are composite organisms found throughout temperate terrestrial forests, with species-specific associations with industrial air pollution. Metagenomic analysis of lichen samples requires robust nucleic acid extraction methodology, a process that is challenging due to the protective cortex layers, high polysaccharide content, and the vast diversity of the internal microbiome. Our method includes physical lysis through garnet bead beating, chemical lysis using a sodium dodecyl sulfate buffer, phenol:chloroform:isoamyl alcohol extraction, and ethanol precipitation. The method was tested on three different lichen samples from two distinct species and yielded metagenomic DNA suitable for sequencing and PCR amplification. This procedure addresses the issues associated with DNA extraction from lichen using common laboratory equipment and reagents without the utilization of liquid nitrogen. This paper presents a cost-effective and accessible DNA extraction method for obtaining high-quality genetic material from dried and preserved lichen specimens. [Display omitted] • DNA extraction from lichens is challenging due to the protective outer cortex,diversity, and polysaccharide content. • High-quality genetic material can be obtained from lichen without the use of liquid nitrogen. • Our protocol extracts DNA from diverse microorganisms in dried lichens, including fungi, algae, bacteria, and viruses. [ABSTRACT FROM AUTHOR]

Published

2024

2. Mycobacterium tuberculosis complex sample processing by mechanical lysis, an essential step for reliable whole genome sequencing.

Author

Hermans, Noud, de Zwaan, Rina, Mulder, Arnout, van den Dool, Joyce, van Soolingen, Dick, Kremer, Kristin, and Anthony, Richard

Subjects

*WHOLE genome sequencing, *MYCOBACTERIUM tuberculosis, *TURNAROUND time, *DNA sequencing, *SAMPLING (Process)

Abstract

Mycobacterium tuberculosis complex (MTBC) whole genome sequencing (WGS) turnaround time and WGS success rates are highly influenced by DNA extraction protocols even from cultures. Efficient mycobacterial lysis is crucial for obtaining sufficient DNA from cultures to facilitate reliable genomic drug susceptibility prediction and accurate genotyping with WGS. We compared four DNA extraction protocols from BD BACTEC™ Mycobacterial Growth Indicator Tubes (MGIT) for WGS with a focus on the lysis step: protocol A) column-based protocol without mechanical lysis; protocol B) an adapted protocol including a bead beating step; protocol C) DNA extraction from primary received cultures using bead beating: and protocol D) DNA extraction from pre MGIT-positive (enriched) cultures. Protocol B increased DNA yield approximately 60-fold, and significantly improved the sequencing success rate. The increased yield also allowed DNA extraction from primary cultures with high success rates (protocol C). Additionally, by using pre-positive enriched MGIT cultures, we demonstrated that bead beating opens the possibility of reliable WGS up to five days before a MGIT tube would be flagged positive (protocol D). The most optimal bead beating-based DNA extraction was also evaluated for Nanopore sequencing. Shortening bead beating duration to 15 s resulted in longer read lengths (N50 from 1.4 kb to 2.6 kb) while still providing efficient lysis. Furthermore, AmpureXP bead beating-based DNA capture / purification proved to be as efficient as Qiagen column-based DNA extraction, further simplifying and shortening the DNA extraction protocol. Adding a mechanical lysis step to our routine MTBC DNA extraction protocol has allowed us to reduce the turnaround time while maintaining DNA quality sequencing success rates. • Bead beating improves DNA yield from M. tuberculosis complex 60-fold. • Mechanical lysis simplifies DNA extraction dramatically reducing turnaround time. • Optimized bead beating protocols can result in DNA suitable for long read sequencing. [ABSTRACT FROM AUTHOR]

Published

2024

3. Technical and economic efficiency of methods for extracting genomic DNA from Meloidogyne javanica.

Author

Carvalho, Vanessa Rafaela de, Wilcken, Sílvia Renata Siciliano, Wilcken, Carlos Frederico, Castro, Bárbara Monteiro de Castro e, Soares, Marcus Alvarenga, and Zanuncio, José Cola

Subjects

*GENOMICS, *JAVANESE root-knot nematode, *PLANT nematodes, *NEMATODES, *NUCLEIC acid isolation methods

Abstract

Abstract Plant parasitic nematodes reduce the production of agricultural crops. Species diagnosis is essential to predict losses, determine economic damage levels and develop integrated pest management programs. DNA extraction techniques need to be improved for precise and rapid molecular diagnosis of nematodes. The objective of the present study was to evaluate the efficiency of DNA extraction and amplification by PCR, cost and execution time by Chelex, Worm Lysis Buffer Method (WLB), Holterman Lysis Buffer Method (HLB) and FastDNA methods for nematodes of the Meloidogyne genus. The qualitative and quantitative efficiency of DNA extraction varied between methods. The band size of the amplified PCR product with WLB, Chelex and HLB methods was 590 bp. Extraction with the FastDNA is not recommended for DNA extraction from nematodes because it results in a low DNA concentration without bands in PCR amplification, besides presenting high cost. The efficiency of the WLB method to extracting DNA from Meloidogyne javanica was greater, ensuring a higher concentration and purity of the extracted material and guaranteeing lower costs and greater ease of PCR amplification. Highlights • Extraction with the FastDNA is not recommended for DNA extraction from nematodes. • WLB is more efficient to extract DNA from M. javanica that Chelex and HLB methods. • Extraction with WLB method has lower cost and better PCR amplification. [ABSTRACT FROM AUTHOR]

Published

2019

4. Comparison of freeze-thaw cycles for nucleic acid extraction and molecular detection of Cryptosporidium parvum and Toxoplasma gondii oocysts in environmental matrices.

Author

Manore, Anna J.W., Harper, Sherilee L., Aguilar, Beatriz, Weese, J.S., and Shapiro, Karen

Subjects

*FREEZE-thaw cycles, *NUCLEIC acid analysis, *DETACHMENT reactions, *CRYPTOSPORIDIUM parvum, *TOXOPLASMA gondii

Abstract

Abstract Freeze-thaw DNA extraction methods and PCR primers were compared to optimize detection of Cryptosporidium parvum and Toxoplasma gondii oocysts in different matrices. Increasing FT cycles did not increase parasite DNA detection, and primers targeting the 18S ssrRNA gene yielded the most sensitive detection of C. parvum oocysts. Highlights • Increasing Freeze-thaw (FT) cycles did not enhance parasite DNA extraction. • Toxoplasma gondii was detected in mussel tissue and water following one FT cycle. • Cryptosporidium parvum detection was highest targeting the 18S ssrRNA gene. [ABSTRACT FROM AUTHOR]

Published

2019

5. Evaluation of DNA extraction methods to detect bacterial targets in aerosol samples.

Author

Dunbar, John, Gallegos-Graves, La Verne, Gans, Jason, Morse, Stephen A., Pillai, Segaran, Anderson, Kevin, and Hodge, David R.

Subjects

*BACTERIAL cells, *AEROSOLS, *NUCLEIC acid isolation methods, *PATHOGENIC bacteria, *MICROBIAL ecology, *BACTERIAL DNA

Abstract

Abstract DNA-based monitoring of pathogens in aerosol samples requires extraction methods that provide high recovery of DNA. To identify a suitable method, we evaluated six DNA extraction methods for recovery of target-specific DNA from samples with four bacterial agents at low abundance (<10,000 genome copies per detection assay). These methods differed in rigor of cell disruption, approach for DNA capture, and extent of DNA purification. The six methods varied 1000-fold in the recovery of DNA from spores or cells of surrogates of Bacillus anthracis, Yersinia pestis, Burkholderia pseudomallei, and Francisella tularensi s, each at about 105 CFU per sample. A custom method using paramagnetic Dynabeads for DNA capture greatly outperformed the other five methods. The cDynabead method provided about 80% recovery of target-specific DNA. The cDynabead method and a filtration method were further evaluated for DNA recovery from bacterial agents spiked on filters (c.a. 105 CFU of each agent per filter quadrant) that were subsequently used to collect background outdoor air particulates for 24-h. The filtration method generally failed to recover detectable quantities of target DNA from the spiked filters, suggesting at least a 100-fold loss of target DNA during extraction, whereas the custom cDynabead method consistently yielded DNA sufficient for target detection. Highlights • The performance of DNA extraction methods with low quantities of material is not routinely evaluated. • Among six methods, we found one dramatically outperformed the rest with relatively low quantities of target material. • This finding is a valuable performance benchmark for a broad range of environmental microbiology applications. [ABSTRACT FROM AUTHOR]

Published

2018

6. Comparison of DNA extraction methods for drug susceptibility testing by allele-specific primer extension on a microsphere-based platform: Chelex-100 (in-house and commercialized) and MagPurix TB DNA Extraction Kit.

Author

Kang, Minji, Yang, Jeong Seong, Kim, Yoojeong, Kim, Kyungjong, Choi, Hongjo, and Lee, Seung Heon

Subjects

*NUCLEIC acid isolation methods, *TUBERCULOSIS diagnosis, *MICROSPHERES, *GENETIC mutation, *MICROBIAL sensitivity tests, *MYCOBACTERIUM tuberculosis

Abstract

Abstract Tuberculosis (TB), caused by infections of the Mycobacterium tuberculosis (MTB) complex, is the ninth leading cause of death worldwide, and several molecular approaches for MTB species identification and the detection of mutations associated with drug resistance have been developed to date. We previously developed a diagnostic assay for drug susceptibility testing that can detect mutations conferring resistance to anti-TB drugs using allele-specific primer extension on a microsphere-based platform for multiplex polymerase chain reaction. The aim of the present study was to optimize this diagnostic assay based on the evaluation of three methods for extracting mycobacterial DNA from clinical samples. Mycobacterial DNA of 81 samples was digested and decontaminated by N -acetyl- l -cysteine-2% NaOH and then extracted using three methods: "in-house" 5% Chelex-100 chelating resin, InstaGene Matrix, and MagPurix TB DNA Extraction Kit. The former two methods are manual extraction methods, whereas the MagPurix TB DNA Extraction Kit is an automated extraction method used with the MagPurix 12 s automated nucleic acid purification system. The extracted DNA was then subjected to our diagnostic assay, and the results were compared among methods. The magnetic bead method exhibited a higher extraction efficiency and resulted in greater diagnostic efficacy than the two resin-based methods with respect to both target gene detection and acid-fast bacilli smear grades. Therefore, the MagPurix TB DNA Extraction Kit is the optimal MTB DNA extraction method for our diagnostic assay of TB drug susceptibility testing. Highlights • Magnetic beads extract DNA of greater purity than that extracted by resin. • Magnetic bead DNA extraction had higher efficiency in detection of TB genes. • The automated extraction system is technically simple and completely closed. • Magnetic bead extraction is optimal for anti-TB drug susceptibility gene testing. [ABSTRACT FROM AUTHOR]

Published

2018

7. Comparison of three DNA extraction methods for molecular confirmation of Mycobacterium avium subspecies paratuberculosis from the VersaTrek™ liquid cultures of bovine fecal samples.

Author

Thirumalapura, Nagaraja R., Feria, Willard, and Tewari, Deepanker

Subjects

*MYCOBACTERIUM avium paratuberculosis, *PARATUBERCULOSIS, *MICROBIAL cultures, *POLYETHYLENE glycol, *NUCLEIC acid isolation methods, *DIAGNOSIS

Abstract

Abstract We evaluated three DNA extraction methods for confirmation of Mycobacterium avium subspecies paratuberculosis from liquid cultures of bovine feces. Use of DNA Extract All Reagents Kit™ resulted in efficient extraction of amplifiable DNA from higher proportion (96.29%) of known positive samples compared to Chelex-100 resin (25.92%) and polyethylene glycol (0%). Highlights • Johne's disease is caused by Mycobacterium avium subsp. paratuberculosis (MAP). • PCR is used for confirmation of MAP in liquid cultures for the disease diagnosis. • Use of DNA Extract All Reagents Kit™ resulted in efficient extraction of MAP DNA. [ABSTRACT FROM AUTHOR]

Published

2018

8. Two efficient methods for isolation of high-quality genomic DNA from entomopathogenic fungi.

Author

Serna-Domínguez, María G., Andrade-Michel, Gilda Y., Arredondo-Bernal, Hugo C., and Gallou, Adrien

Subjects

*NUCLEIC acid isolation methods, *ENTOMOPATHOGENIC fungi, *LIQUID nitrogen, *METABOLITES, *POLYMERASE chain reaction

Abstract

Conventional and commercial methods for isolation of nucleic acids are available for fungal samples including entomopathogenic fungi (EPF). However, there is not a unique optimal method for all organisms. The cell wall structure and the wide range of secondary metabolites of EPF can broadly interfere with the efficiency of the DNA extraction protocol. This study compares three commercial protocols: DNeasy® Plant Mini Kit (Qiagen), Wizard® Genomic DNA Purification Kit (Promega), and Axygen™ Multisource Genomic DNA Miniprep Kit (Axygen) and three conventional methods based on different buffers: SDS, CTAB/PVPP, and CTAB/β-mercaptoethanol versus three cell lysis procedures: liquid nitrogen homogenization and two bead-beating materials (i.e., tungsten-carbide and stainless-steel) for four representative species of EPF (i.e., Beauveria bassiana , Hirsutella citriformis , Isaria javanica , and Metarhizium anisopliae ). Liquid nitrogen homogenization combined with DNeasy® Plant Mini Kit (i.e., QN) or SDS buffer (i.e., SN) significantly improved the yield with a good purity (~1.8) and high integrity (>20,000 bp) of genomic DNA in contrast with other methods, also, these results were better when compared with the two bead-beating materials. The purified DNA was evaluated by PCR-based techniques: amplification of translation elongation factor 1-α (TEF) and two highly sensitive molecular markers (i.e., ISSR and AFLP) with reliable and reproducible results. Despite a variation in yield, purity, and integrity of extracted DNA across the four species of EPF with the different DNA extraction methods, the SN and QN protocols maintained a high-quality of DNA which is required for downstream molecular applications. [ABSTRACT FROM AUTHOR]

Published

2018

9. Comparison of ten different DNA extraction procedures with respect to their suitability for environmental samples.

Author

Kuhn, Ramona, Böllmann, Jörg, Krahl, Kathrin, Bryant, Isaac Mbir, and Martienssen, Marion

Subjects

*DNA analysis, *NUCLEIC acid isolation methods, *ULTRAVIOLET spectrophotometry, *FLUORESCENCE spectroscopy, *WASTEWATER treatment

Abstract

DNA extraction for molecular biological applications usually requires target optimized extraction procedures depending on the origin of the samples. For environmental samples, a range of different procedures has been developed. We compared the applicability and efficiency of ten selected DNA extraction methods published in recent literature using four different environmental samples namely: activated sludge from a domestic wastewater treatment plant, river sediment, anaerobic digestion sludge and nitrifying enrichment culture. We assessed the suitability of the extraction procedures based on both DNA yield and quality. DNA quantification was performed by both ultra violet (UV) spectrophotometry and fluorescence spectrophotometry after staining with PicoGreen. In our study, DNA yields based on UV measurement were overestimated in most cases while DNA yields from fluorescence measurements correlated well with the sample load on agarose gels of crude DNA. The quality of the DNA extracts was determined by gel electrophoresis of crude DNA and PCR products from 16S rDNA with the universal primer set 27f/1525r. It was observed that gel electrophoresis of crude DNA was not always suitable to evaluate DNA integrity and purity since interfering background substances (e.g. humic substances) were not visible. Therefore, we strongly recommend examining the DNA quality of both crude DNA and 16S rDNA PCR products by gel electrophoresis when a new extraction method is established. Summarizing, we found four out of ten extraction procedures being applicable to all tested samples without noticeable restrictions. The procedure G (according to the standard method 432_10401 of the Lower Saxony State Office for Consumer Protection and Food Safety) had the broadest application range over procedure J (published by Wilson, 2001). These were followed by procedures F (Singka et al., 2012) and A (Bourrain et al., 1999). All four extraction procedures delivered reliable and reproducible crude DNA and PCR products. From an economical point of view, all procedures tested during this study were cheaper compared to commercial DNA extraction kits. [ABSTRACT FROM AUTHOR]

Published

2017

10. Assessing impacts of DNA extraction methods on next generation sequencing of water and wastewater samples.

Author

Walden, Connie, Carbonero, Franck, and Zhang, Wen

Subjects

*NUCLEIC acid isolation methods, *GENETIC techniques, *SEWAGE, *LAKES, *BIOFILMS

Abstract

Next Generation Sequencing (NGS) is increasingly affordable and easier to perform. However, standard protocols prior to the sequencing step are only available for few selected sample types. Here we investigated the impact of DNA extraction methods on the consistency of NGS results. Four commercial DNA extraction kits (QIAamp DNA Mini Kit, QIAamp DNA Stool Mini Kit, MO BIO Power Water Kit, and MO BIO Power Soil DNA Isolation Kit) were used on sample sources including lake water and wastewater, and sample types including planktonic and biofilm bacteria communities. Sampling locations included a lake water reservoir, a trickling filter, and a moving bed biofilm reactor (MBBR). Unique genera such as Gemmatimonadetes , Elusimicrobia , and Latescibacteria were found in multiple samples. The Stool Mini Kit was least efficient in terms of diversity in sampling results with freshwater lake samples, and surprisingly the Power Water Kit was the least efficient across all sample types examined. Detailed NGS beta diversity comparisons indicated that the Mini Kit and PowerSoil Kit are best suited for studies that extract DNA from a variety of water and wastewater samples. We ultimately recommend application of Mini Kit or PowerSoil Kit as an improvement to NGS protocols for these sampling environments. These results are a step toward achieving accurate comparability of complex samples from water and wastewater environments by applying a single DNA extraction method, further streamlining future investigations. [ABSTRACT FROM AUTHOR]

Published

2017

11. Improved method for rapid and accurate isolation and identification of Streptococcus mutans and Streptococcus sobrinus from human plaque samples.

Author

Villhauer, Alissa L., Lynch, David J., and Drake, David R.

Subjects

*DIAGNOSIS of dental caries, *STREPTOCOCCUS mutans, *DISEASE progression, *GLYCOSYLTRANSFERASES, *NUCLEIC acid isolation methods

Abstract

Mutans streptococci (MS), specifically Streptococcus mutans (SM) and Streptococcus sobrinus (SS), are bacterial species frequently targeted for investigation due to their role in the etiology of dental caries. Differentiation of S. mutans and S. sobrinus is an essential part of exploring the role of these organisms in disease progression and the impact of the presence of either/both on a subject's caries experience. Of vital importance to the study of these organisms is an identification protocol that allows us to distinguish between the two species in an easy, accurate, and timely manner. While conducting a 5-year birth cohort study in a Northern Plains American Indian tribe, the need for a more rapid procedure for isolating and identifying high volumes of MS was recognized. We report here on the development of an accurate and rapid method for MS identification. Accuracy, ease of use, and material and time requirements for morphological differentiation on selective agar, biochemical tests, and various combinations of PCR primers were compared. The final protocol included preliminary identification based on colony morphology followed by PCR confirmation of species identification using primers targeting regions of the glucosyltransferase ( gtf ) genes of SM and SS. This method of isolation and identification was found to be highly accurate, more rapid than the previous methodology used, and easily learned. It resulted in more efficient use of both time and material resources. [ABSTRACT FROM AUTHOR]

Published

2017

12. Evaluation of the Punch-it™ NA-Sample kit for detecting microbial DNA in blood culture bottles using PCR-reverse blot hybridization assay.

Author

Kim, Jungho, Wang, Hye-young, Kim, Seoyong, Park, Soon Deok, Yu, Kwangmin, Kim, Hyo Youl, Uh, Young, and Lee, Hyeyoung

Subjects

*NUCLEIC acid isolation methods, *DNA analysis, *POLYMERASE chain reaction, *NUCLEIC acid hybridization, *PAPER chromatography, *BLOOD sampling

Abstract

DNA extraction efficiency affects the success of PCR-based method applications. The Punch-it™ NA-Sample kit for extracting DNA by using paper chromatography is technically easy to use and requires just two reagents and only 10 min to complete. The Punch-it™ NA-Sample kit could be offered as a rapid, accurate, and convenient method for extracting bacterial and fungal DNA from blood culture bottles. We compared the efficiencies of the commercial kit (Punch-it™ NA-Sample kit) and an in-house conventional boiling method with Chelex-100 resin for DNA extraction from blood culture bottles. The efficiency of the two DNA extraction methods was assessed by PCR-reverse blot hybridization assay (PCR-REBA, REBA Sepsis-ID) for detecting Gram positive (GP) bacteria, Gram negative (GN) bacteria, and Candida species with 196 positive and 200 negative blood culture bottles. The detection limits of the two DNA extraction methods were 10 3 CFU/mL for GP bacteria, 10 3 CFU/mL for GN bacteria, and 10 4 CFU/mL for Candida . The sensitivity and specificity of the Punch-it™ NA-Sample kit by REBA Sepsis-ID were 95.4% (187/196) and 100% (200/200), respectively. The overall agreement of the two DNA extraction methods was 98.9% (392/396). Three of four samples showing discrepant results between the two extraction methods were more accurately matched up with the Punch-it™ NA-Sample kit based on conventional culture methods. The results indicated that the Punch-it™ NA-Sample kit extracted bacterial and fungal DNA in blood culture bottles and allowed extracted DNA to be used in molecular assay. [ABSTRACT FROM AUTHOR]

Published

2016

13. Comparison of four commercial DNA extraction kits for the recovery of Bacillus spp. spore DNA from spiked powder samples.

Author

Mölsä, Markos, Kalin-Mänttäri, Laura, Tonteri, Elina, Hemmilä, Heidi, and Nikkari, Simo

Subjects

*NUCLEIC acid isolation methods, *BACILLUS anthracis, *ANTHRAX, *BACILLUS thuringiensis, *DNA analysis

Abstract

Bacillus spp. include human pathogens such as Bacillus anthracis , the causative agent of anthrax and a biothreat agent. Bacillus spp. form spores that are physically highly resistant and may remain active over sample handling. We tested four commercial DNA extraction kits (QIAamp DNA Mini Kit, RTP Pathogen Kit, ZR Fungal/Bacterial DNA MiniPrep, and genesig Easy DNA/RNA Extraction kit) for sample inactivation and DNA recovery from two powders (icing sugar and potato flour) spiked with Bacillus thuringiensis spores. The DNA was analysed using a B. thuringiensis -specific real-time PCR assay. The detection limit was 3 × 10 1 CFU of spiked B. thuringiensis spores with the QIAamp DNA Mini, RTP Pathogen, and genesig Easy DNA/RNA Extraction kits, and 3 × 10 3 CFU with the ZR Fungal/Bacterial DNA MiniPrep kit. The results showed that manual extraction kits are effective and safe for fast and easy DNA extraction from powder samples even in field conditions. Adding a DNA filtration step to the extraction protocol ensures the removal of Bacillus spp. spores from DNA samples without affecting sensitivity. [ABSTRACT FROM AUTHOR]

Published

2016

14. Optimization of subculture and DNA extraction steps within the whole genome sequencing workflow for source tracking of Salmonella enterica and Listeria monocytogenes.

Author

Gimonet, Johan, Portmann, Anne-Catherine, Fournier, Coralie, and Baert, Leen

Subjects

*NUCLEIC acid isolation methods, *NUCLEOTIDE sequencing, *SALMONELLA enterica, *WATER gas shift reactions, *SINGLE nucleotide polymorphisms

Abstract

This work shows that an incubation time reduced to 4–5 h to prepare a culture for DNA extraction followed by an automated DNA extraction can shorten the hands-on time, the turnaround time by 30% and increase the throughput while maintaining the WGS quality assessed by high quality Single Nucleotide Polymorphism analysis. [ABSTRACT FROM AUTHOR]

Published

2018

15. Alkaline treatment of resting spores prior to DNA extraction improves the purity of Plasmodiophora brassicae DNA.

Author

Yang, Yalong, Zahr, Kher, Harding, Michael W., Strelkov, Stephen E., Zuzak, Krista, Feindel, David, and Feng, Jie

Subjects

*PLASMODIOPHORA brassicae, *SPORES, *DNA contamination, *HOST plants, *PLANT cells & tissues

Abstract

A commonly used protocol for DNA extraction from Plasmodiophora brassicae was modified by adding an alkaline treatment step to increase the purity of resting spores. The quality of DNA extracted by the modified protocol was improved due to the removal of DNA contamination from host plant cells and other microorganisms. [ABSTRACT FROM AUTHOR]

Published

2018

16. Selenite enrichment broth to improve the sensitivity in molecular diagnostics of Salmonella

Author

Maria Dullaert-de Boer, Adri G. M. van der Zanden, Elles Sterne, Richard F. de Boer, Annel Lameijer, Anita W.M. Suijkerbuijk, Max Heck, and Ben Skidmore

Subjects

DNA, Bacterial, Microbiology (medical), Salmonella, Enrichment broth, chemistry.chemical_element, Selenious Acid, medicine.disease_cause, Polymerase Chain Reaction, Sensitivity and Specificity, Microbiology, Feces, 03 medical and health sciences, Multiplexed real-time PCR, medicine, Humans, Molecular Biology, 030304 developmental biology, 0303 health sciences, biology, 030306 microbiology, Outbreaks, Salmonella enterica, biology.organism_classification, Molecular diagnostics, DNA extraction, Culture Media, Gastroenteritis, Foodborne disease, Fecal coliform, chemistry, Salmonella Infections, Selenite enrichment, Selenium

Abstract

Selenite enrichment broth (SEB) is used to optimize the recovery of Salmonella enterica subspecies enterica from stool samples. Compared to a direct culture approach, it enhances culture yield by reducing growth of faecal coliforms and faecal streptococci. Over the course of seven years from 2000 to 2017, 47,235 faecal samples were tested with a Salmonella PCR. We investigated the added value of using SEB in combination with faeces for DNA extraction, in order to improve the sensitivity of molecular diagnostics for detection of Salmonella. A Salmonella enterica subspecies enterica strain was tested for growth characteristics, with and without incubation in SEB, to determine the impact of Selenite enrichment in the Salmonella PCR. Retrospectively, a total of 102 Salmonella enterica subspecies enterica PCR positive faecal samples were re-analysed. DNA extraction was performed with the EasyMag® and MagNaPure96® system using three different input volumes of faeces and SEB. Prospectively, 114 Salmonella PCR positive faecal samples were retested within 2 days using five different input volumes for DNA extraction. Retrospectively, PCR that used SEB as part of input in the DNA extraction, 7/102 (7%) Salmonella PCR positive samples were additionally detected compared to no use of SEB. Of these, Salmonella enterica subspecies enterica serovariation Thompson, Enteritidis, 9,12:l.v and Senftenberg have been outbreak related in the past. Prospectively results were combined in collaboration with another microbiology laboratory, 15/114 (13.2%) additional specimens were detected with the Salmonella PCR, including processing Selenite enrichment broth. In conclusion, of the total 47,235 feacal samples, with SEB the prevalence of a positive PCR for Salmonella is 2.2%. Of these 2.2% positive Salmonella PCRs, 0.4% was not detected in culture. By using SEB an improved detection of Salmonella diagnostics could be realized and a substantial part of 13,2% additional Salmonella cases could be detected.

Published

2019

17. New rapid DNA extraction method with Chelex from Venturia inaequalis spores.

Author

Turan, Ceren, Nanni, Irene Maja, Brunelli, Agostino, and Collina, Marina

Subjects

*NUCLEIC acid isolation methods, *VENTURIA inaequalis, *DNA analysis, *POLYMERASE chain reaction, *COMPARATIVE studies

Abstract

The objective of this study was to develop a rapid method to isolate DNA from Venturia inaequalis spores for use in diagnostic DNA mutation analysis. Chelex-100 resin was evaluated and compared with a well established DNA exctraction method, utilizing CTAB in order to have a robust comparison. In this research we demonstrated that Chelex-100 efficiently makes extraction of the DNA from V. inaequalis spores available for direct use in molecular analyses. Also, the quantity and quality of extracted DNA were shown to be adequate for PCR analysis. Comparatively, the quality of DNA samples isolated using Chelex method was better than those extracted using CTAB. In conclusion, the Chelex method is recommended for PCR experiments considering its simplicity and cost-effectiveness. [ABSTRACT FROM AUTHOR]

Published

2015

18. Microbial food safety: Potential of DNA extraction methods for use in diagnostic metagenomics.

Author

Josefsen, Mathilde H., Andersen, Sandra C., Christensen, Julia, and Hoorfar, Jeffrey

Subjects

*FOOD microbiology, *NUCLEIC acid isolation methods, *METAGENOMICS, *FOOD safety, *CAMPYLOBACTER jejuni, *POLYMERASE chain reaction

Abstract

The efficiency of ten widely applied DNA extraction protocols was evaluated for suitability for diagnostic metagenomics. The protocols were selected based on a thorough literature study. Chicken fecal samples inoculated with about 1 × 10 3 and 1 × 10 6 CFU/g Campylobacter jejuni were used as a model. The evaluation was performed based on total DNA yield measured by fluorometry, and quality and quantity of C. jejuni DNA measured by real-time PCR. There was up to a 25-fold variance between the lowest (NucliSens miniMAG, BIOMÉRIEUX) and highest (PowerLyzer PowerSoil DNA Isolation Kit, MO BIO Laboratories) yielding protocols. The PowerLyzer PowerSoil DNA Isolation Kit performed significantly better than all other protocols tested. Selected protocols were modified, i.e., extended heating and homogenization, resulting in increased yields of total DNA. For QIAamp Fast DNA Stool Mini Kit (Qiagen) a 7-fold increase in total DNA was observed following the protocol for human DNA analysis and including a 5 min heating step at 70 °C. For the PowerLyzer PowerSoil and the PowerFecal DNA Isolation Kit (MO BIO Laboratories) the total DNA fold increase was 1.6 to 1.8 when including an extra 10 min of bead-vortexing. There was no correlation between the yield of total DNA and the amount of PCR-amplifiable DNA from C. jejuni . The protocols resulting in the highest yield of total DNA did not show correspondingly increased levels of C. jejuni DNA as determined by PCR. In conclusion, substantial variation in the efficiency of the protocols to extract DNA was observed. The highest DNA yield was obtained with the PowerLyzer PowerSoil DNA Isolation Kit, whereas the FastDNA SPIN Kit for Feces (MP Biomedicals) resulted in the highest amount of PCR-amplifiable C. jejuni DNA. [ABSTRACT FROM AUTHOR]

Published

2015

19. A review on application of next-generation sequencing methods for profiling of protozoan parasites in water: Current methodologies, challenges, and perspectives

Author

Isaac Dennis Amoah, Nonsikelelo Precios Mthethwa, Faizal Bux, Sheena Kumari, and Poovendhree Reddy

Subjects

Microbiology (medical), Computer science, Computational biology, Microbiology, DNA, Ribosomal, DNA sequencing, Specimen Handling, 03 medical and health sciences, Eukaryotic genome, Animals, Parasites, Molecular Biology, 030304 developmental biology, Profiling (computer programming), 0303 health sciences, 030306 microbiology, Computational Biology, High-Throughput Nucleotide Sequencing, Water, Water current, Sequence Analysis, DNA, DNA, Protozoan, DNA extraction, Workflow, Key factors, Metagenomics, Metagenome, Parasitology

Abstract

The advancement in metagenomic techniques has provided novel tools for profiling human parasites in environmental matrices, such as water and wastewater. However, application of metagenomic techniques for the profiling of protozoan parasites in environmental matrices is not commonly reported in the literature. The key factors leading to the less common use of metagenomics are the complexity and large eukaryotic genome, the prevalence of small parasite populations in environmental samples compared to bacteria, difficulties in extracting DNA from (oo)cysts, and limited reference databases for parasites. This calls for further research to develop optimized methods specifically looking at protozoan parasites in the environment. This study reviews the current workflow, methods and provide recommendations for the standardization of techniques. The article identifies and summarizes the key methods, advantages, and limitations associated with metagenomic analysis, like sample pre-processing, DNA extraction, sequencing approaches, and analysis methods. The study enhances the understanding and application of standardized protocols for profiling of protozoan parasite community from highly complexe samples and further creates a resourceful comparison among datasets without any biases.

Published

2021

20. Fast and automated detection of common carbapenemase genes using multiplex real-time PCR on the BD MAX™ system

Author

Michael Bandilla, Alexander H. Dalpke, Sébastien Boutin, Katja Probst, and Klaus Heeg

Subjects

Microbiology (medical), DNA, Bacterial, Bacilli, Reference laboratory, Real-Time Polymerase Chain Reaction, Microbiology, Sensitivity and Specificity, beta-Lactamases, 03 medical and health sciences, Bacterial Proteins, Germany, Multiplex polymerase chain reaction, Humans, Multiplex, Molecular Biology, Gene, 030304 developmental biology, 0303 health sciences, biology, Bacteria, 030306 microbiology, Rectum, biology.organism_classification, Molecular diagnostics, DNA extraction, Virology, Anti-Bacterial Agents, Real-time polymerase chain reaction, Molecular Diagnostic Techniques, Multiplex Polymerase Chain Reaction

Abstract

Fast detection of carbapenemases in Gram-negative bacilli is necessary for accurate antibiotic treatment, prevention of further spreading and surveillance purposes. We analyzed the current occurrence of gene variants and designed two multiplex PCRs with hydrolysis probes. The assay was developed for the BD MAX™ system that combines DNA extraction and PCR in a fully automated procedure providing results within 3 h and was evaluated for detection of carbapenemases from bacterial isolates and directly from rectal swabs. The assay has a theoretic coverage of 97.1% for carbapenemases detected during the last years by the German National Reference Laboratory (NRL). A collection of 151 isolates from the NRL was used and all carbapenemase-positive bacteria (58/58) were identified correctly. The direct-PCR on rectal swabs revealed additional carbapenemase genes in 7 samples that were not identified by the culture-based method used as reference method. The assay allows detection of carbapenemases from clinical isolates and might also help in rapid detection directly from rectal samples.

Published

2021

21. Evaluation of a commercial microbial enrichment kit used prior DNA extraction to improve the molecular detection of vector-borne pathogens from naturally infected dogs

Author

Chayan Roy, Melody Koo, Kristina M. Oney, Brian B. Oakley, Nicholas B. Juhasz, Barbara A. Qurollo, Songyang Ren, Pedro Diniz, and Elton J R Vasconcelos

Subjects

Microbiology (medical), DNA, Bacterial, Ehrlichia ewingii, Anaplasma, Ehrlichia, Vector Borne Diseases, Parasitemia, Biology, Real-Time Polymerase Chain Reaction, Microbiology, Polymerase Chain Reaction, DNA sequencing, chemistry.chemical_compound, Dogs, RNA, Ribosomal, 16S, medicine, RNA, Ribosomal, 18S, Animals, Dog Diseases, Molecular Biology, Tick-borne disease, Bacteria, Microbiota, High-Throughput Nucleotide Sequencing, DNA, Protozoan, medicine.disease, biology.organism_classification, Molecular diagnostics, DNA extraction, Real-time polymerase chain reaction, chemistry, Tick-Borne Diseases, DNA, Anaplasma phagocytophilum

Abstract

Accurate detection of vector-borne pathogens (VBPs) is extremely important as the number of reported cases in humans and animals continues to rise in the US and abroad. Validated PCR assays are currently the cornerstone of molecular diagnostics and can achieve excellent analytical sensitivity and specificity. However, the detection of pathogens at low parasitemia still presents a challenge for VBP diagnosis, especially given the very low volume of specimens tested by molecular methods. The objective of this study is to determine if a commercially available microbial enrichment kit, used prior DNA extraction , is capable of expanding the overall microbial community and increasing detectable levels of VBPs in canine blood samples through host DNA depletion. This study used EDTA-whole blood samples from dogs naturally infected with varying parasitemia levels of either Anaplasma phagocytophilum , Babesia gibsoni , or Ehrlichia ewingii . For two VBPs, EDTA-blood samples were diluted to determine the effect of microbial concentration at low parasitemia. Paired EDTA-blood samples from each dog were subjected to traditional, automated DNA extraction with or without the microbial concentrating kit (MolYsis®) prior DNA extraction. Relative amounts of pathogen DNA in paired samples were determined by real-time PCR and Next-Generation Sequencing targeting conserved regions of 16S rRNA (for bacteria) and 18S rRNA (for protozoa). Results from the three molecular methods suggest that the microbial concentrating kit did not improve the detection of VBPs, although significantly reduced the presence of host DNA. Alternative methods for VBP enrichment in clinical samples prior to molecular testing should continue to be investigated, as it may significantly improve clinical sensitivity and reduce the number of false-negative results.

Published

2020

22. Comparison of seven methods for extraction of bacterial DNA from fecal and cecal samples of mice.

Author

Ferrand, Janina, Patron, Kevin, Legrand-Frossi, Christine, Frippiat, Jean-Pol, Merlin, Christophe, Alauzet, Corentine, and Lozniewski, Alain

Subjects

*BACTERIAL DNA, *NUCLEIC acid isolation methods, *FECAL analysis, *GENE targeting, *LABORATORY mice, *COMPARATIVE studies, *POLYMERASE chain reaction, *RIBOSOMAL DNA

Abstract

Analysis of bacterial DNA from fecal samples of mice is commonly performed in experimental studies. Although DNA extraction is a critical step in various molecular approaches, the efficiency of methods that may be used for DNA extraction from mice fecal samples has never been evaluated. We compared the efficiencies of six widely used commercial kits (MasterPure™ Gram Positive DNA Purification Kit, QIAamp® DNA Stool Mini Kit; NucliSENS® easyMAG®, ZR Fecal DNA MiniPrep™, FastDNA® SPIN Kit for Feces and FastDNA® SPIN Kit for Soil) and a non-commercial method for DNA isolation from mice feces and cecal contents. DNA quantity and quality were assessed by fluorometry, spectrophotometry, gel electrophoresis and qPCR. Cell lysis efficiencies were evaluated by qPCR targeting three relevant bacteria in spiked specimens. For both feces and intestinal contents, the most efficient extraction method was the FastDNA® SPIN Kit for Soil. [ABSTRACT FROM AUTHOR]

Published

2014

23. An optimized DNA extraction protocol for benthic Didymosphenia geminata.

Author

Uyua, Noelia Mariel, Manrique, Julieta Marina, and Jones, Leandro Roberto

Subjects

*NUCLEIC acid isolation methods, *DIATOMS, *POLYSACCHARIDES, *HEAVY metals, *BENTHIC ecology, *POLYMERASE chain reaction

Abstract

Didymosphenia geminata mats display few cells in relation to extracellular material and contain polysaccharides and heavy metals that interfere with molecular studies. We describe an optimized DNA extraction protocol that help to overcome these difficulties. Our protocol outperformed five previously described DNA extraction techniques. [ABSTRACT FROM AUTHOR]

Published

2014

24. Isolation of PCR quality microbial community DNA from heavily contaminated environments.

Author

Gunawardana, Manjula, Chang, Simon, Jimenez, Abraham, Holland-Moritz, Daniel, Holland-Moritz, Hannah, La Val, Taylor P., Lund, Craig, Mullen, Madeline, Olsen, John, Sztain, Terra A., Yoo, Jennifer, Moss, John A., and Baum, Marc M.

Subjects

*POLYMERASE chain reaction, *MICROBIAL contamination, *DNA, *ASPHALT, *BIODEGRADATION, *BIOMASS energy, *HYDROPHILIC compounds, *RIBOSOMAL RNA

Abstract

Abstract: Asphalts, biochemically degraded oil, contain persistent, water-soluble compounds that pose a significant challenge to the isolation of PCR quality DNA. The adaptation of existing DNA purification protocols and commercial kits proved unsuccessful at overcoming this hurdle. Treatment of aqueous asphalt extracts with a polyamide resin afforded genomic microbial DNA templates that could readily be amplified by PCR. Physicochemically distinct asphalt samples from five natural oil seeps successfully generated the expected 291bp amplicons targeting a region of the 16S rRNA gene, illustrating the robustness of the method. DNA recovery yields were in the 50–80% range depending on how the asphalt sample was seeded with exogenous DNA. The scope of the new method was expanded to include soil with high humic acid content. DNA from soil samples spiked with a range of humic acid concentrations was extracted with a commercial kit followed by treatment with the polyamide resin. The additional step significantly improved the purity of the DNA templates, especially at high humic acid concentrations, based on qPCR analysis of the bacterial 16S rRNA genes. The new method has the advantages of being inexpensive, simple, and rapid and should provide a valuable addition to protocols in the field of petroleum and soil microbiology. [Copyright &y& Elsevier]

Published

2014

25. Evaluation of MolYsis™ Complete5 DNA extraction method for detecting Staphylococcus aureus DNA from whole blood in a sepsis model using PCR/pyrosequencing.

Author

McCann, Chase D. and Jordan, Jeanne A.

Subjects

*NUCLEIC acid isolation methods, *STAPHYLOCOCCUS aureus, *BACTERIAL DNA, *POLYMERASE chain reaction, *SEPSIS, *COMPARATIVE studies

Abstract

Abstract: Bacterial bloodstream infections (BSI) and ensuing sepsis are important causes of morbidity and mortality. Early diagnosis and rapid treatment with appropriate antibiotics are vital for improving outcome. Nucleic acid amplification of bacteria directly from whole blood has the potential of providing a faster means of diagnosing BSI than automated blood culture. However, effective DNA extraction of commonly low levels of bacterial target from whole blood is critical for this approach to be successful. This study compared the Molzyme MolYsis™ Complete5 DNA extraction method to a previously described organic bead-based method for use with whole blood. A well-characterized Staphylococcus aureus-induced pneumonia model of sepsis in canines was used to provide clinically relevant whole blood samples. DNA extracts were assessed for purity and concentration and analyzed for bacterial rRNA gene targets using PCR and sequence-based identification. Both extraction methods yielded relatively pure DNA with median A260/280 absorbance ratios of 1.71 (MolYsis™) and 1.97 (bead-based). The organic bead-based extraction method yielded significantly higher average DNA concentrations (P<0.05) at each time point throughout the experiment, closely correlating with changes observed in white blood cell (WBC) concentrations during this same time period, while DNA concentrations of the MolYsis™ extracts closely mirrored quantitative blood culture results. Overall, S. aureus DNA was detected from whole blood samples in 70.7% (58/82) of MolYsis™ DNA extracts, and in 59.8% (49/82) of organic bead-based extracts, with peak detection rates seen at 48h for both MolYsis™ (87.0%) and organic bead-based (82.6%) methods. In summary, the MolYsis™ Complete5 DNA extraction kit proved to be the more effective method for isolating bacterial DNA directly from extracts made from whole blood. [Copyright &y& Elsevier]

Published

2014

26. Versatile broad-host-range cosmids for construction of high quality metagenomic libraries.

Author

Cheng, Jiujun, Pinnell, Lee, Engel, Katja, Neufeld, Josh D., and Charles, Trevor C.

Subjects

*NOCTUIDAE, *METAGENOMICS, *GENE libraries, *COSMIDS, *PROTEOBACTERIA, *MOLECULAR cloning, *GENETIC vectors

Abstract

Abstract: We constructed IncP broad-host-range Gateway® entry cosmids pJC8 and pJC24, which replicate in diverse Proteobacteria. We demonstrate the functionality of these vectors by extracting, purifying, and size-selecting metagenomic DNA from agricultural corn and wheat soils, followed by cloning into pJC8. Metagenomic DNA libraries of 8×104 (corn soil) and 9×106 (wheat soil) clones were generated for functional screening. The DNA cloned in these libraries can be transferred from these recombinant cosmids to Gateway® destination vectors for specialized screening purposes. Those library clones are available from the Canadian MetaMicroBiome Library project (http://www.cm2bl.org/). [Copyright &y& Elsevier]

Published

2014

27. Clinical evaluation of an automated Real-Prep system for extracting nucleic acids to detect mycobacterial infection

Author

Chae Hoon Lee, Hyung Woo Kim, and Jong Ho Lee

Subjects

Microbiology (medical), Adult, DNA, Bacterial, Male, Bodily Secretions, Adolescent, Respiratory System, Real-Time Polymerase Chain Reaction, Microbiology, Mycobacterium, Specimen Handling, Mycobacterium tuberculosis, 03 medical and health sciences, chemistry.chemical_compound, Young Adult, medicine, Humans, Molecular Biology, 030304 developmental biology, Aged, Aged, 80 and over, 0303 health sciences, Mycobacterium Infections, Chromatography, biology, 030306 microbiology, Chemistry, Extraction (chemistry), Middle Aged, biology.organism_classification, DNA extraction, Manual extraction, Nucleic acid, Sputum, Female, medicine.symptom, Clinical evaluation, DNA

Abstract

Real-time PCR tests have been widely used to detect mycobacterial infection. The quality of extracted DNA is crucial for obtaining accurate results of the real-time PCR tests, and automated extraction methods are faster and more effective than manual extraction. The novel Real-Prep automated extraction system has not yet been verified by direct comparisons to existing methods. In this study, we compared it with manual extraction, and the Nextractor system, an automated extraction method commonly used in Korea. From August to December 2018, 238 specimens, including sputum, bronchial washing, pericardial fluid, bronchial aspiration, pleural fluid, and closed pus samples, were collected and examined at Yeungnam University Hospital. After decontamination, smear microscopy, and culturing, DNA was extracted using the three methods. The DNA extraction efficiency (total amount of DNA [ng]/input specimen volume [μL]) and purity (A260/280 ratio), which indicates the presence of contaminants, were compared. Real-time PCR tests were conducted using the DNA extracted by each method. The cycle threshold, which is inversely related to the initial amount of mycobacterial DNA, and the percentage agreement between the PCR results of the three methods were evaluated. Our study revealed that the DNA extraction efficiency of the Real-Prep system was higher than that of manual extraction. There was no significant difference in DNA purity between the methods, and the percentage agreement for Mycobacterium tuberculosis and non-tuberculous mycobacteria among all three methods was almost perfect. The performance of the Real-Prep system was similar to that of the Nextractor system and superior to that of manual extraction. The Real-Prep system, a new automated nucleic acid extraction device, has a clear benefit because of its relative speed and low hands-on time. Therefore, the Real-Prep system is a useful substitute for manual DNA extraction, which has the potential to reduce workloads in laboratories and as a sensitive non-tuberculous mycobacteria detection method throughout the world.

Published

2020

28. PCR-based quantification of taxa-specific abundances in microbial communities: Quantifying and avoiding common pitfalls

Author

Denny Popp, Fabian Bonk, Florian Centler, and Hauke Harms

Subjects

DNA, Bacterial, 0301 basic medicine, Microbiology (medical), Bacteria, Microbiota, 030106 microbiology, High-Throughput Nucleotide Sequencing, Computational biology, Models, Theoretical, Biology, Amplicon, Real-Time Polymerase Chain Reaction, Microbiology, DNA extraction, Genome, DNA sequencing, 03 medical and health sciences, 030104 developmental biology, Taxon, Species Specificity, RNA, Ribosomal, 16S, Amplicon sequencing, Critical assessment, Molecular Biology, Genome, Bacterial

Abstract

The quantification of relative and absolute taxa-specific abundances in complex microbial communities is crucial for understanding and modeling natural and engineered ecosystems. Many errors inherent to this quantification are, though well-known, still insufficiently addressed and can potentially lead to a completely different interpretation of experimental results. This review provides a critical assessment of next generation sequencing (NGS) of amplicons and quantitative real-time PCR for the quantification of relative and absolute taxa-specific genome abundances. Starting from DNA extraction, the following error sources were considered: DNA extraction efficiency, PCR-associated bias, variance of strain-specific 16S rRNA operon copy number per genome, and analysis of quantitative real-time PCR and NGS data. Tools and methods for estimating and minimizing these errors are presented and demonstrated on published data. In conclusion, amplicon sequencing and qPCR of 16S rRNA genes are valuable tools to determine relative and absolute taxa-specific genome abundances, but results can deviate by several orders of magnitudes from the true values if the reviewed error sources are ignored. Many of these errors can be minimized in a cost-efficient manner and large errors can be easily identified by plausibility checks as shown in this review. Finally, the accurate conversion of genome abundances to cell numbers and microbial biomasses was pointed out as an important future research topic for the integration of PCR-based abundances into mathematical models.

Published

2018

29. Optimisation of protocol for effective detachment and selective recovery of the representative bacteria for extraction of metagenomic DNA from Eucalyptus spp. woodchips

Author

Chika F. Nnadozie, Johnson Lin, and Roshini Govinden

Subjects

DNA, Bacterial, 0301 basic medicine, Microbiology (medical), Sonication, 030106 microbiology, Microbiology, law.invention, Matrix (chemical analysis), 03 medical and health sciences, chemistry.chemical_compound, law, Molecular Biology, Filtration, Eucalyptus, Chromatography, Bacteria, biology, Chemistry, Extraction (chemistry), biology.organism_classification, Wood, DNA extraction, Woodchips, Metagenomics, Stress, Mechanical, DNA

Abstract

For some environments such as planktonic/aqueous environments, the separation of bacteria cells from eukaryotic cells prior to DNA extraction using filtration is relatively straightforward. However, for woodchips, the bacteria are attached/embedded within the wood matrix, which prevents easy removal of bacterial cells. In this study, a method for the selective extraction of DNA from bacteria inhabiting Eucalyptus spp. woodchips has been developed. The objective was to compare milled and unmilled woodchips processed via three detachment methods, viz., sonication, vortexing and shaking followed by filtration using Teflon filters according to three relevant criteria: DNA yield, DNA purity and quality of DNA. Highest DNA yield was obtained by milling and vortexing for 10 min (77.50 ± 5.17 ng/μl), followed by milling and vortexing for 2 min (61.00 ± 6.56 ng/μl), unmilled and vortexing for 10 min (38.67 ± 5.17 ng/μl) and milled and shaking for 2 h (31.62 ± 5.17 ng/μl). The lowest DNA yield was obtained by using unmilled woodchips and 5 min of sonication treatment (7.00 ± 1.22 ng/μl). There was no significant difference in DNA purity for milled or unmilled woodchips processed via the three detachment methods. Duration of cell detachment treatment did not significantly influence DNA yield and purity. Following optimisation experiments, it was possible to extract bacterial DNA using milled woodchips and 10 minute vortexing devoid of DNA from the host background and other associated eukaryotes and of sufficient quality and quantity for metagenomic analysis.

Published

2018

30. Analysis of DNA extraction methods for detection of Treponema pallidum: A comparison of three methods

Author

Maria Lucia Rosa Rossetti, Márcia Susana Nunes Silva, Mauro Cunha Ramos, Liliane Trivellato Grassi, and Vera Mileide Trivellato Grassi

Subjects

DNA, Bacterial, Male, Microbiology (medical), Sexually transmitted disease, Lipoproteins, Biology, Sensitivity and Specificity, Microbiology, chemistry.chemical_compound, medicine, Humans, Syphilis, Treponema pallidum, Molecular Biology, Gene, Chromatography, Treponema, Base Sequence, Sequence Analysis, DNA, medicine.disease, biology.organism_classification, DNA extraction, Molecular analysis, genomic DNA, chemistry, Nucleic Acid Amplification Techniques, DNA

Abstract

Syphilis is a sexually transmitted disease caused by Treponema pallidum . DNA amplification methods have started to be used to facilitate diagnosis at different stages of the disease. The success of such methodologies depends on obtaining DNA from clinical samples in adequate quantity and quality for molecular reactions. There are many DNA extraction kits, but often the molecular analysis process is unfeasible due to its cost and access to imported products. Thus, this study aimed to analyze three methods of extracting DNA from Treponema pallidum from ulcers of patients investigated for syphilis. The three methods, an in house one (sonication) and two commercial ones (LGC, Brazil) and the PureLink Genomic DNA Mini Kit (Thermo Fisher Scientific, USA) were compared to the sequencing of these samples, which were used as a reference. Each method was evaluated based on the detection of T. pallidum by PCR using the tpp47 gene as a target for amplification, DNA quantification and method execution time. When compared to the sequencing, the sensitivity and agreement of the PureLink, sonication and LGC methods to extracted DNA were 100% (K = 1.0), 96.5% (K = 0.96) and 72.4% (K = 0.694), respectively. Specificity was 100% with the three methods. The sonication method was the closest in concentration of DNA to the PureLink method with a similar degree of purity, besides having the lowest cost-benefit ratio. It can be an interesting option for laboratories that work with reduced costs, since it is much more financially viable.

Published

2022

31. Simultaneous quantitation of 3ADON and 15ADON chemotypes of DON-producing Fusarium species in Chinese wheat based on duplex droplet digital PCR assay

Author

Meng Ze Chen, Song Shan Wang, Yu Wu, Song Xue Wang, Li Li, and Hua Cui

Subjects

Microbiology (medical), Fusarium, China, Veterinary medicine, Genotype, Chemotype, biology, Trichothecene, food and beverages, biology.organism_classification, Polymerase Chain Reaction, Microbiology, DNA extraction, Geographic distribution, Fusariosis, Duplex (building), Yangtze river, Digital polymerase chain reaction, DNA, Fungal, Trichothecenes, Molecular Biology, Triticum, Plant Diseases

Abstract

Pathogens within Fusarium species are the primary agents of Fusarium head blight (FHB) of wheat, which bring about yield reduction and deoxynivalenol (DON) contamination and are of great concern worldwide. DON-producing Fusarium species can be classified into 3-acetyldeoxynivalenol (3ADON) and 15-acetyldeoxynivalenol (15ADON) chemotypes according to the trichothecene metabolites they produce. The detection of these two chemotypes of pathogens is paramount to the successful implementation of disease management strategies and pathogen-related DON forecasting models. In this study, a duplex droplet digital PCR (duplex ddPCR) assay was developed that allowed for the simultaneous quantitation of 3ADON and 15ADON chemotypes of DON-producing Fusarium species. The assay specificity was tested against 30 isolates of target Fusarium species and several non-target Fusarium species that are frequently isolated from wheat in China. Analyzing 90 wheat samples collected from the North China plain and Yangtze River plain demonstrated that the duplex ddPCR assay coupled with magnetic bead-based DNA extraction was competent for investigating composition of 3ADON and 15ADON chemotypes in Chinese wheat. This assay will be useful for monitoring the epidemic and geographic distribution of 3ADON and 15ADON chemotypes of FHB pathogens, which will help with the disease control and DON management.

Published

2021

32. Comparison of direct boiling method with commercial kits for extracting fecal microbiome DNA by Illumina sequencing of 16S rRNA tags.

Author

Peng, Xin, Yu, Ke-Qiang, Deng, Guan-Hua, Jiang, Yun-Xia, Wang, Yu, Zhang, Guo-Xia, and Zhou, Hong-Wei

Subjects

*DNA, *RIBOSOMAL RNA, *BIOLOGICAL tags, *NUCLEOTIDE sequence, *ENVIRONMENTAL sciences, *NUCLEIC acid isolation methods, *METAGENOMICS

Abstract

Abstract: Low cost and high throughput capacity are major advantages of using next generation sequencing (NGS) techniques to determine metagenomic 16S rRNA tag sequences. These methods have significantly changed our view of microorganisms in the fields of human health and environmental science. However, DNA extraction using commercial kits has shortcomings of high cost and time constraint. In the present study, we evaluated the determination of fecal microbiomes using a direct boiling method compared with 5 different commercial extraction methods, e.g., Qiagen and MO BIO kits. Principal coordinate analysis (PCoA) using UniFrac distances and clustering showed that direct boiling of a wide range of feces concentrations gave a similar pattern of bacterial communities as those obtained from most of the commercial kits, with the exception of the MO BIO method. Fecal concentration by boiling method affected the estimation of α-diversity indices, otherwise results were generally comparable between boiling and commercial methods. The operational taxonomic units (OTUs) determined through direct boiling showed highly consistent frequencies with those determined through most of the commercial methods. Even those for the MO BIO kit were also obtained by the direct boiling method with high confidence. The present study suggested that direct boiling could be used to determine the fecal microbiome and using this method would significantly reduce the cost and improve the efficiency of the sample preparation for studying gut microbiome diversity. [Copyright &y& Elsevier]

Published

2013

33. A comparison of the efficiency of five different commercial DNA extraction kits for extraction of DNA from faecal samples.

Author

Claassen, Shantelle, du Toit, Elloise, Kaba, Mamadou, Moodley, Clinton, Zar, Heather J., and Nicol, Mark P.

Subjects

*NUCLEIC acid isolation methods, *GUT microbiome, *FECES, *MICROBIOLOGY, *POLYMERASE chain reaction, *GEL electrophoresis, *RESTRICTION fragment length polymorphisms, *BACTERIAL diversity, *DNA denaturation

Abstract

Differences in the composition of the gut microbiota have been associated with a range of diseases using culture-independent methods. Reliable extraction of nucleic acid is a key step in identifying the composition of the faecal microbiota. Five widely used commercial deoxyribonucleic acid (DNA) extraction kits (QIAsymphony® Virus/Bacteria Midi Kit (kit QS), ZR Fecal DNA MiniPrep™ (kit Z), QIAamp® DNA Stool Mini Kit (kit QA), Ultraclean® Fecal DNA Isolation Kit (kit U) and PowerSoil® DNA Isolation Kit (kit P)) were evaluated, using human faecal samples. Yield, purity and integrity of total genomic DNA were compared spectrophotometrically and using gel electrophoresis. Three bacteria, commonly found in human faeces were quantified using real time polymerase chain reaction (qPCR) and total bacterial diversity was studied using denaturing gradient gel electrophoresis (DGGE) as well as terminal restriction fragment length polymorphism (T-RFLP). The measurements of DNA yield and purity exhibited variations between the five kits tested in this study. Automated kit QS exhibited the best quality and highest quantity of DNA. All kits were shown to be reproducible with CV values≤0.46 for DNA extraction. qPCR results showed that all kits were uniformly efficient for extracting DNA from the selected target bacteria. DGGE and T-RFLP produced the highest diversity scores for DNA extracted using kit Z (H′=2.30 and 1.27) and kit QS (H′=2.16 and 0.94), which also extracted the highest DNA yields compared to the other kits assessed. [ABSTRACT FROM AUTHOR]

Published

2013

34. Quantification of Cryptosporidium parvum in natural soil matrices and soil solutions using qPCR

Author

Koken, Emre, Darnault, Christophe J.G., Jacobson, Astrid R., Powelson, David, and Hendrickson, William

Subjects

*CRYPTOSPORIDIUM parvum, *SOIL solutions, *POLYMERASE chain reaction, *MICROSCOPY, *SOIL matric potential, *ETHYLENEDIAMINETETRAACETIC acid, *LYSIS, *OOCYSTS, *DNA

Abstract

Abstract: Traditional microscopy methods for the detection and quantification of Cryptosporidium parvum in soil matrices are time-consuming, labor-intensive, and lack sensitivity and specificity. This research focused on developing a qPCR protocol for the sensitive and specific detection and quantification of C. parvum in natural soil matrices and soil–water extracts. The physico-chemical parameters — lysis media, number of thermal shocks and thawing temperatures — controlling DNA extraction efficiency were investigated. Experimental results identified oocyst age as a critical parameter affecting oocyst disruption and quantification. The most efficient oocyst disruption method for C. parvum oocysts regardless of their age was established as 5 thermal shocks with thawing at 65°C in Tris-EDTA (TE) buffer. In addition to the purification columns used to remove PCR inhibitors present in environmental matrices, a combination of 3mM MgCl2 and 600ng/μl BSA yielded the highest amplicon yield for both young and aged oocysts. Sucrose flotation was determined to be a better oocyst isolation method than two-phase flotation. The optimized parameters for DNA extraction and the qPCR assay resulted in very specific and sensitive detection of C. parvum. Minimum detection limits were 0.667 for young C. parvum oocysts and 6.67 for aged C. parvum oocysts per PCR reaction. The accuracy of the detections and quantifications was 0.999. Protocol performance was tested in contrasting soil samples and soil–water extract samples on the basis of percentage of recovery (PR) values. Depending on the number of oocysts used to inoculate the samples, the average PR values ranged from 7.2 to 43.5%, 29.3–52.5%, and 11.5–60.8% for Trenton, Greenson, and Sparta soil–water extracts, respectively, and 12.1–77% for DI water. PR values ranged from 4.3% to 107.8% for Trenton, Greenson and Sparta soil samples. [Copyright &y& Elsevier]

Published

2013

35. Assessment of three commercial DNA extraction kits and a laboratory-developed method for detecting Cryptosporidium and Cyclospora in raspberry wash, basil wash and pesto

Author

Shields, Joan M., Joo, Jane, Kim, Richard, and Murphy, Helen R.

Subjects

*CRYPTOSPORIDIUM, *PARASITIC insects, *GENETIC markers, *RASPBERRIES, *PROTOZOA, *RIBOSOMAL RNA, *NUCLEIC acid separation, *POLYMERASE chain reaction

Abstract

Abstract: Polymerase chain reaction (PCR) methods are often used to identify the parasitic protozoa Cryptosporidium parvum and Cyclospora cayetanensis in foods although little has been published regarding the efficacy of available DNA extraction methods. This study reviewed three commonly used commercial DNA extraction kits: FastDNA SPIN Kit for soil, QBiogene (FastDNA), UltraClean™ Soil DNA Isolation Kit, MO BIO Laboratories (MoBio), and QIAamp DNA Mini Stool Kit, Qiagen (QIAamp), as well as a ‘homebrew’ Universal Nucleic Acid Extraction (UNEX) method. Washes from raspberry and basil as well as commercial pesto samples were seeded with 5000, 500, or 50 C. parvum and C. cayetanensis oocysts. The protocols were assessed for: quantity and quality of the extracted DNA, time to completion, presence of PCR inhibitors and the percentage of samples correctly identified as positive for the two parasites. Real-time and conventional nested PCR assays were used to detect the seeded pathogens. Of the commercial kits, PCR results of samples extracted using FastDNA were statistically similar to QIAamp and both were superior to MoBio. Differences in PCR results among FastDNA, QIAamp and UNEX for detection of Cyclospora were not statistically significant although the UNEX method proved best with Cryptosporidium. Real-time PCR assays targeted the 18S rRNA and the hsp70 genes of C. cayetanensis; overall results were similar to those found using conventional nested PCR targeting the 18S rRNA gene. [Copyright &y& Elsevier]

Published

2013

36. DNA extractions from deep subseafloor sediments: Novel cryogenic-mill-based procedure and comparison to existing protocols

Author

Alain, Karine, Callac, Nolwenn, Ciobanu, Maria-Cristina, Reynaud, Yann, Duthoit, Frédérique, and Jebbar, Mohamed

Subjects

*DNA, *ENZYME inhibitors, *BIOMASS, *SEDIMENTS, *LOW temperature engineering, *LIQUID nitrogen, *PROKARYOTES, *CHLOROFORM

Abstract

Abstract: Extracting DNA from deep subsurface sediments is challenging given the complexity of sediments types, low biomasses, resting structures (spores, cysts) frequently encountered in deep sediments, and the potential presence of enzymatic inhibitors. Promising results for cell lysis efficiency were recently obtained by use of a cryogenic mill (Lipp et al., 2008). These findings encouraged us to devise a DNA extraction protocol using this tool. Thirteen procedures involving a combination of grinding in liquid nitrogen (for various durations and beating rates) with different chemical solutions (phenol, chloroform, SDS, sarkosyl, proteinase, GTC), or with use of DNA recovery kits (MagExtractor®) were compared. Effective DNA extraction was evaluated in terms of cell lysis efficiency, DNA extraction efficiency, DNA yield and determination of prokaryotic diversity. Results were compared to those obtained by standard protocols: the FastDNA®SPIN kit for soil and the Zhou protocol. For most sediment types grinding in a cryogenic mill at a low beating rate in combination with direct phenol-chloroform extraction resulted in much higher DNA yields than those obtained using classical procedures. In general (except for clay-rich sediments), this procedure provided high-quality crude extracts for direct downstream nested-PCR, from cell numbers as low as 1.1×106 cells/cm3. This procedure is simple, rapid, low-cost, and could be used with minor modifications for large-scale DNA extractions for a variety of experimental goals. [Copyright &y& Elsevier]

Published

2011

37. Metagenomic comparison of direct and indirect soil DNA extraction approaches

Author

Delmont, Tom O., Robe, Patrick, Clark, Ian, Simonet, Pascal, and Vogel, Timothy M.

Subjects

*GENOMES, *DNA, *PRAIRIES, *METABOLISM, *MICROBIOLOGY, *STATISTICAL bootstrapping, *BIODIVERSITY, *CONFIDENCE intervals

Abstract

Abstract: Full pyrosequencing runs of both direct-extracted (high yield, low DNA size) and indirect-extracted DNA (low yield, high DNA size) from the same prairie soil show that the sequence distribution of the majority of the metabolic functions and species detected were statistically similar. Although some microbial functions differed at the 95% confidence interval in bootstrap analyses, the overall functional diversity was the same. [Copyright &y& Elsevier]

Published

2011

38. Comparative analysis of fecal DNA extraction methods with phylogenetic microarray: Effective recovery of bacterial and archaeal DNA using mechanical cell lysis

Author

Salonen, Anne, Nikkilä, Janne, Jalanka-Tuovinen, Jonna, Immonen, Outi, Rajilić-Stojanović, Mirjana, Kekkonen, Riina A., Palva, Airi, and de Vos, Willem M.

Subjects

*COMPARATIVE studies, *MOLECULAR phylogeny, *POLYMERASE chain reaction, *ENZYMATIC analysis, *RNA, *BIOTIC communities, *BACTERIAL diversity, *ARCHAEBACTERIA

Abstract

Abstract: Several different protocols are used for fecal DNA extraction, which is an integral step in all phylogenetic and metagenomic approaches to characterize the highly diverse intestinal ecosystem. We compared four widely used methods, and found their DNA yields to vary up to 35-fold. Bacterial, archaeal and human DNA was quantified by real-time PCR, and a compositional analysis of different extracts was carried out using the Human Intestinal Tract Chip, a 16S rRNA gene-based phylogenetic microarray. The overall microbiota composition was highly similar between the methods in contrast to the profound differences between the subjects (Pearson correlations >0.899 and 0.735, respectively). A detailed comparative analysis of mechanical and enzymatic methods showed that despite their overall similarity, the mechanical cell disruption by repeated bead beating showed the highest bacterial diversity and resulted in significantly improved DNA extraction efficiency of archaea and some bacteria, including Clostridium cluster IV. By applying the mechanical disruption method a high prevalence (67%) of methanogenic archaea was detected in healthy subjects (n =24), exceeding the typical values reported previously. The assessment of performance differences between different methodologies serves as a concrete step towards the comparison and reliable meta-analysis of the results obtained in different laboratories. [Copyright &y& Elsevier]

Published

2010

39. An efficient DNA isolation protocol for filamentous cyanobacteria of the genus Arthrospira

Author

Morin, Nicolas, Vallaeys, Tatiana, Hendrickx, Larissa, Natalie, Leys, and Wilmotte, Annick

Subjects

*CYANOBACTERIA, *NUCLEIC acid separation, *DIETARY supplements, *BIOMASS energy, *SPACE flight, *MOLECULAR cloning, *POLYMERASE chain reaction, *MOLECULAR biology, *BACTERIAL genomes

Abstract

Abstract: Thanks to their photosynthetic and nutritive properties, cyanobacteria of the Arthrospira genus are of interest as food supplements, as efficient oxygen producing life support system organisms for manned space flight, and for the production of biofuels. Despite these potential valuable applications, full genome sequences and genetic information in general on Arthrospira remain scarce. This is mainly due to the difficulty to extract sufficient high molecular weight nucleic acids from these filamentous cyanobacteria. In this article, an efficient and reproducible DNA extraction procedure for cyanobacteria of the genus Arthrospira was developed. The method is based on the combination of a soft mechanical lysis with enzymatic disruption of the cell wall. The comparison with other extraction protocols clearly indicates that this optimised method allows the recovery of a larger amount of DNA. Furthermore, the extracted DNA presents a high molecular weight, a reduced degradation and an excellent overall quality. It can be directly used for molecular biology purposes such as PCR, and clone library construction. [Copyright &y& Elsevier]

Published

2010

40. Evaluation of a modified rapid viability-polymerase chain reaction method for Bacillus atrophaeus spores in water matrices

Author

Rebecca N. Bushon, Amie M.G. Brady, Christopher M. Kephart, and Vicente J. Gallardo

Subjects

DNA, Bacterial, Microbiology (medical), Sample (material), Ultrafiltration, chemistry.chemical_element, Bacillus, Polymerase Chain Reaction, Sensitivity and Specificity, Microbiology, Article, Tap water, Chlorine, Centrifugation, Molecular Biology, Spores, Bacterial, Bacteriological Techniques, Microbial Viability, Chromatography, biology, Water, biology.organism_classification, DNA extraction, Spore, chemistry, Bacillus atrophaeus, Water Microbiology

Abstract

A rapid method that provides information on the viability of organisms is needed to protect public health and ensure that remediation efforts following a release of a biological agent are effective. The rapid viability-polymerase chain reaction (RV-PCR) method combines broth culture and molecular methods to provide results on whether viable organisms are present in less than 15 h. In this study, a modified RV-PCR (mRV-PCR) method was compared to a membrane-filtration culture method for the detection of viable Bacillus spores in water matrices. Samples included small and large volumes of chlorine and non‑chlorine treated tap water. Large volume water samples (up to 100 L), were processed by ultrafiltration using a semi-automated waterborne pathogen concentrator, followed by centrifugation as a secondary concentration technique. The concentrated samples were analyzed by mRV-PCR and culture methods. The overall agreement between the mRV-PCR and culture methods when seed concentrations were greater than 10 spores per sample volume analyzed was 96%. The total time from the start of sample processing to the final sample result for the mRV-PCR method was decreased by approximately 2 h, in comparison to the previously published RV-PCR method because of the incorporation of shorter, more efficient primary and secondary concentration steps and a shorter DNA extraction technique. Overall, this study confirmed that RV-PCR is a promising approach for identifying viable Bacillus spores in small- and large-volume water samples and for producing results in less time than traditional culture methods.

Published

2021

41. Field preservation and DNA extraction methods for intestinal microbial diversity analysis in earthworms

Author

Thakuria, Dwipendra, Schmidt, Olaf, Liliensiek, Ann-Kathrin, Egan, Damian, and Doohan, Fiona M.

Subjects

*GUT microbiome, *MICROBIAL diversity, *EARTHWORMS, *MICROBIOLOGICAL techniques, *NUCLEOTIDE sequence, *DNA fingerprinting, *SPECTROPHOTOMETRY, *POLYMERASE chain reaction

Abstract

Abstract: We assessed the effect of DNA extraction and sample preservation methods on the DNA yield and quality obtained from earthworm (Aporrectodea caliginosa Savigny) gut samples and on the results obtained by bacterial and fungal automated ribosomal intergenic spacer analysis (ARISA) of DNA extracts. Methods based on a hexadecyltrimethylammonium bromide dithiotreitol (CTAB-DTT) extraction buffer yielded more favourable results than those based on a sodium dodecyl sulphate (SDS) buffer. For both of these buffers, incorporation of a bead-beating during the lysis step increased the ARISA-derived bacterial ribotype numbers and diversity estimates, as determined for gut wall samples (P <0.01). Although spectrophotometric analysis indicated that DNA extracted by the CTAB-DTT and SDS-based methods were of comparable quality (P ≥0.05), the former method yielded >1.5 times more DNA from both gut contents and gut walls of earthworms than the latter method (both incorporating the bead beating step) (P <0.01). ARISA analysis detected more reproducible ribotypes and more microbial diversity in DNA extracted by the CTAB-DTT- as compared to the SDS-based method (P <0.01). Significant difference between bacterial communities of gut contents and gut walls were detected within DNA extracted by the CTAB-DTT (but not by the SDS-based) method (Global R =0.76, P <0.001, analysis of similarity). Using the CTAB-DTT-based method, we showed that earthworm preservation in ethanol yielded higher quality DNA from gut contents than preservation in either chloroform or liquid N, as determined by spectrophotometry, PCR inhibition analysis and bacterial and fungal ARISA (P <0.05). Bacterial or fungal communities in the gut contents of fresh and ethanol-preserved earthworms were more similar and were significantly different from those of earthworms preserved in chloroform or liquid N (Global R =0.79 and 0.83 for bacteria and fungi, respectively; P <0.001, analysis of similarity). We propose that ethanol preservation and the CTAB-DTT-based DNA extraction method described herein are also suitable for the analysis of gut-associated microbiota in other soil and sediment feeding invertebrates. [Copyright &y& Elsevier]

Published

2009

42. A comparison of DNA extraction procedures for the detection of Mycobacterium ulcerans, the causative agent of Buruli ulcer, in clinical and environmental specimens

Author

Durnez, Lies, Stragier, Pieter, Roebben, Karen, Ablordey, Anthony, Leirs, Herwig, and Portaels, Françoise

Subjects

*NUCLEOTIDE sequence, *DNA, *MYCOBACTERIUM, *BACTERIAL typing, *ULCERS, *MYCOBACTERIAL diseases, *POLYMERASE chain reaction, *COMPARATIVE studies

Abstract

Abstract: Mycobacterium ulcerans is the causative agent of Buruli ulcer, the third most common mycobacterial disease in humans after tuberculosis and leprosy. Although the disease is associated with aquatic ecosystems, cultivation of the bacillus from the environment is difficult to achieve. Therefore, at the moment, research is based on the detection by PCR of the insertion sequence IS2404 present in M. ulcerans and some closely related mycobacteria. In the present study, we compared four DNA extraction methods for detection of M. ulcerans DNA, namely the one tube cell lysis and DNA extraction procedure (OT), the FastPrep procedure (FP), the modified Boom procedure (MB), and the Maxwell® 16 Procedure (M16). The methods were performed on serial dilutions of M. ulcerans, followed by PCR analysis with different PCR targets in M. ulcerans to determine the detection limit (DL) of each method. The purity of the extracted DNA and the time and effort needed were compared as well. All methods were performed on environmental specimens and the two best methods (MB and M16) were tested on clinical specimens for detection of M. ulcerans DNA. When comparing the DLs of the DNA extraction methods, the MB and M16 had a significantly lower DL than the OT and FP. For the different PCR targets, IS2404 showed a significantly lower DL than mlsA, MIRU1, MIRU5 and VNTR6. The FP and M16 were considerably faster than the MB and OT, while the purity of the DNA extracted with the MB was significantly higher than the DNA extracted with the other methods. The MB performed best on the environmental and clinical specimens. This comparative study shows that the modified Boom procedure, although lengthy, provides a better method of DNA extraction than the other methods tested for detection and identification of M. ulcerans in both clinical and environmental specimens. [Copyright &y& Elsevier]

Published

2009

43. Molecular detection of Puccinia horiana in Chrysanthemum x morifolium through conventional and real-time PCR

Author

Alaei, Hossein, Baeyen, Steve, Maes, Martine, Höfte, Monica, and Heungens, Kurt

Subjects

*PUCCINIA, *CHRYSANTHEMUM diseases & pests, *FUNGAL diseases of plants, *POLYMERASE chain reaction, *EXTRACTION (Chemistry), *PLANT clones, *PATHOGENIC fungi

Abstract

Abstract: Puccinia horiana Henn. is a quarantine organism and one of the most important fungal pathogens of Chrysanthemum x morifolium cultivars grown for cut flower or potted plant production (florist''s chrysanthemum) in several regions of the world. Highly specific primer pairs were identified for conventional, nested, and real-time PCR detection of P. horiana based on the specific and sensitive PCR amplification of selected regions in the internal transcribed spacers (ITS1 and ITS2) of the nuclear ribosomal DNA (rDNA). Using these different PCR versions, 10 pg, 10 fg, and 5 fg genomic DNA could be detected, respectively. When using cloned target DNA as template, the detection limits were 5000, 50, and 5 target copies, respectively. These detection limits were not affected by a background of chrysanthemum plant DNA. The DNA extraction method was optimized to maximize the recoverability of the pathogen from infected plant tissue. A CTAB extraction protocol or a selection of commercial DNA extraction methods allowed the use of 10 ng total (plant+pathogen) DNA without interference of PCR inhibitors. Due to the specificity of the primers, SYBR Green I technology enabled reliable real time PCR signal detection. However, an efficient TaqMan probe is available. The lowest proportion of infected plant material that could still be detected when mixed with healthy plant material was 0.001%. The real-time PCR assay could detect as few as eight pure P. horiana basidiospores, demonstrating the potential of the technique for aerial detection of the pathogen. The amount of P. horiana DNA in plant tissue was determined at various time points after basidiospore inoculation. Using the real-time PCR protocol, it was possible to detect the pathogen immediately after the inoculation period, even though the accumulation of pathogen DNA was most pronounced near the end of the latent period. The detection system proved to be accurate and sensitive and could help not only in pathogen diagnosis but also in pathogen monitoring and disease forecasting systems. [Copyright &y& Elsevier]

Published

2009

44. Evaluation of five commercial nucleic acid extraction kits for their ability to inactivate Bacillus anthracis spores and comparison of DNA yields from spores and spiked environmental samples

Author

Dauphin, Leslie A., Moser, Benjamin D., and Bowen, Michael D.

Subjects

*BACILLUS anthracis, *NUCLEIC acids, *BACTERIAL spores, *EXTRACTION techniques, *POLYMERASE chain reaction, *BIOTERRORISM, *GENOMICS

Abstract

Abstract: This study evaluated five commercial extraction kits for their ability to recover DNA from Bacillus anthracis spores and spiked environmental samples. The kits evaluated represent the major types of methodologies which are commercially available for DNA or total nucleic acid extraction, and included the ChargeSwitch gDNA Mini Bacteria Kit, NucliSens Isolation Kit, Puregene Genomic DNA Purification Kit, QIAamp DNA Blood Mini Kit, and the UltraClean Microbial DNA Isolation Kit. Extraction methods were performed using the spores of eight virulent strains of B. anthracis. Viability testing of nucleic acid extracts showed that the UltraClean kit was the most efficient at depleting samples of live B. anthracis spores. TaqMan real-time PCR analysis revealed that the NucliSens, QIAamp and UltraClean kits yielded the best level of detection from spore suspensions. Comparisons of processed samples from spiked swabs and three powder types indicated that DNA extraction using the UltraClean kit resulted in the most consistently positive results and the lowest limit of detection. This study demonstrated that different nucleic extraction methodologies, represented here by various commercial extraction kits, differ in their ability to inactivate live B. anthracis spores as well as DNA yield and purity. In addition, the extraction method used can influence the sensitivity of real-time PCR assays for B. anthracis. [Copyright &y& Elsevier]

Published

2009

45. An effective method for isolation of DNA from pig faeces and comparison of five different methods

Author

Tang, Jun-ni, Zeng, Zhi-guang, Wang, Hong-ning, Yang, Tai, Zhang, Peng-ju, Li, Yu-ling, Zhang, An-yun, Fan, Wen-qiao, Zhang, Yi, Yang, Xin, Zhao, Su-jun, Tian, Guo-bao, and Zou, Li-kou

Subjects

*FECES, *MICROBIOLOGY, *SWINE, *POLYMERASE chain reaction, *DETECTION of microorganisms, *NUCLEOTIDE sequence, *BACTERIAL genomes, *GEL electrophoresis

Abstract

Abstract: Polymerase chain reaction (PCR) detection of microorganism in faecal specimens is hampered by poor recovery of DNA and by the presence of PCR inhibitors. In this paper, we describe a new modified method for extracting PCR-quality microbial community DNA from pig faecal samples, which combines the pretreatment with polyformaldehyde, and subsequent DNA lysis in the presence of CTAB, salt, PVP, and β-mercaptoethanol, followed by isolation of nucleic acids using chloroform (no phenol) based protocol. The method resulted in a 1.3- to 11-fold increase in DNA yield when compared to four other widely used methods. Genomic DNA extracted from all five methods was assessed by both agarose gel electrophoresis and polymerase chain reaction for amplification of 16S rDNA specific fragments. The results showed that the improved method represented a reproducible, simple, and rapid technique for routine DNA extraction from faecal specimens and was notably better than using the QIAamp® DNA Stool Mini Kit. [Copyright &y& Elsevier]

Published

2008

46. Fecal collection, ambient preservation, and DNA extraction for PCR amplification of bacterial and human markers from human feces

Author

Nechvatal, Jordan M., Ram, Jeffrey L., Basson, Marc D., Namprachan, Phanramphoei, Niec, Stephanie R., Badsha, Kawsar Z., Matherly, Larry H., Majumdar, Adhip P.N., and Kato, Ikuko

Subjects

*NUCLEIC acids, *FUNGUS-bacterium relationships, *PROKARYOTES, *EPITHELIAL cells

Abstract

Abstract: Feces contain intestinal bacteria and exfoliated epithelial cells that may provide useful information concerning gastrointestinal tract health. Intestinal bacteria that synthesize or metabolize potential carcinogens and produce anti-tumorigenic products may have relevance to colorectal cancer, the second most common cause of cancer deaths in the USA. To facilitate epidemiological studies relating bacterial and epithelial cell DNA and RNA markers, preservative/extraction methods suitable for self-collection and shipping of fecal samples at room temperature were tested. Purification and PCR amplification of fecal DNA were compared after preservation of stool samples in RNAlater (R) or Paxgene (P), or after drying over silica gel (S) or on Whatman FTA cards (W). Comparisons were made to samples frozen in liquid nitrogen (N2). DNA purification methods included Whatman (accompanying FTA cards), Mo-Bio Fecal (MB), Qiagen Stool (QS), and others. Extraction methods were compared for amount of DNA extracted, DNA amplifiable in a real-time SYBR-Green quantitative PCR format, and the presence of PCR inhibitors. DNA can be extracted after room temperature storage for five days from W, R, S and P, and from N2 frozen samples. High amounts of total DNA and PCR-amplifiable Bacteroides spp. DNA (34%±9% of total DNA) with relatively little PCR inhibition were especially obtained with QS extraction applied to R preserved samples (method QS-R). DNA for human reduced folate carrier (SLC19A1) genomic sequence was also detected in 90% of the QS-R extracts. Thus, fecal DNA is well preserved by methods suitable for self-collection that may be useful in future molecular epidemiological studies of intestinal bacteria and human cancer markers. [Copyright &y& Elsevier]

Published

2008

47. Comparative evaluation of in-house manual, and commercial semi-automated and automated DNA extraction platforms in the sample preparation of human stool specimens for a Salmonella enterica 5'-nuclease assay

Author

Schuurman, Tim, de Boer, Richard, Patty, Rachèl, Kooistra-Smid, Mirjam, and van Zwet, Anton

Subjects

*ENTEROBACTERIACEAE, *FOOD poisoning, *SALMONELLA, *PARASITIC plants

Abstract

Abstract: In the present study, three methods (NucliSens miniMAG [bioMérieux], MagNA Pure DNA Isolation Kit III Bacteria/Fungi [Roche], and a silica-guanidiniumthiocyanate {Si-GuSCN-F} procedure for extracting DNA from stool specimens were compared with regard to analytical performance (relative DNA recovery and down stream real-time PCR amplification of Salmonella enterica DNA), stability of the extracted DNA, hands-on time (HOT), total processing time (TPT), and costs. The Si-GuSCN-F procedure showed the highest analytical performance (relative recovery of 99%, S. enterica real-time PCR sensitivity of 91%) at the lowest associated costs per extraction (€ 4.28). However, this method did required the longest HOT (144 min) and subsequent TPT (176 min) when processing 24 extractions. Both miniMAG and MagNA Pure extraction showed similar performances at first (relative recoveries of 57% and 52%, S. enterica real-time PCR sensitivity of 85%). However, when difference in the observed Ct values after real-time PCR were taken into account, MagNA Pure resulted in a significant increase in Ct value compared to both miniMAG and Si-GuSCN-F (with on average +1.26 and +1.43 cycles). With regard to inhibition all methods showed relatively low inhibition rates (< 4%), with miniMAG providing the lowest rate (0.7%). Extracted DNA was stable for at least 1 year for all methods. HOT was lowest for MagNA Pure (60 min) and TPT was shortest for miniMAG (121 min). Costs, finally, were € 4.28 for Si-GuSCN, € 6.69 for MagNA Pure and € 9.57 for miniMAG. [Copyright &y& Elsevier]

Published

2007

48. Exploring microbial diversity in volcanic environments: A review of methods in DNA extraction

Author

Herrera, Aude and Cockell, Charles S.

Subjects

*DNA, *DEOXYRIBOSE, *NUCLEIC acids, *GENES

Abstract

Abstract: The last decade has been marked by a large number of studies focused on understanding the distribution of microorganisms in volcanic environments. These studies are motivated by the desire to elucidate how the geochemically extreme conditions of such environments can influence microbial diversity both on the surface and in the subsurface of the Earth. The exploration of microbial community diversity has generally not relied on culture-dependent methods, but has been carried out using environmental DNA extraction. Because of the large diversity of chemically and physically complex samples, extracting DNA from volcanic environments is technically challenging. In view of the emerging literature, and our own experience in the optimisation of methods for DNA extraction from volcanic materials, it is timely to provide a methodological comparison. This review highlights and discusses new insights and methods published on DNA extraction methods from volcanic samples, considering the different volcanic environments. A description of a recent method for DNA extraction from basalt and obsidian glass rock samples from Iceland is included. Finally, we discuss these approaches in the wider context of modern work to understand the microbial diversity of volcanic environments. [Copyright &y& Elsevier]

Published

2007

49. Optimization of methods for detecting Mycobacterium avium subsp. paratuberculosis in environmental samples using quantitative, real-time PCR

Author

Cook, Kimberly L. and Britt, Jenks S.

Subjects

*MYCOBACTERIUM avium, *PARATUBERCULOSIS, *MYCOBACTERIAL diseases in animals, *DNA

Abstract

Abstract: Detection of Johne''s disease, an enteric infection of cattle caused by Mycobacterium avium subsp. paratuberculosis (M. paratuberculosis), has been impeded by the lack of rapid, reliable detection methods. The goal of this study was to optimize methodologies for detecting M. paratuberculosis in manure from an infected dairy cow or in contaminated soil samples using a quantitative, real-time PCR (QRT-PCR) based analysis. Three different nucleic acid extraction techniques, the efficiency of direct versus indirect sample extraction, and sample pooling were assessed. The limit of detection was investigated by adding dilutions of M. paratuberculosis to soil. Results show that the highest yield (19.4±2.3 μg−1 DNA extract) and the highest copy number of the targeted M. paratuberculosis IS900 sequence (1.3±0.2×108 copies g−1 manure) were obtained with DNA extracted from manure using Qbiogene''s Fast® DNA Spin kit for soil. Pooling ten samples of M. paratuberculosis-contaminated soil improved the limit of detection ten fold (between 20 and 115 M. paratuberculosis cells g−1 soil). Detection was between 65% and 95% higher when samples were extracted directly using bead-beating than when using pre-treatment with cell extraction buffers. The final soil-sampling and extraction regime was applied for detection of M. paratuberculosis in pasture soil after the removal of a M. paratuberculosis culture positive dairy cow. M. paratuberculosis remained in the pasture soil for more than 200 days. Results from these studies suggest that DNA extraction method, sampling protocol and PCR conditions each critically influence the outcome and validity of the QRT-PCR analysis of M. paratuberculosis concentrations in environmental samples. [Copyright &y& Elsevier]

Published

2007

50. Optimization of terminal restriction fragment polymorphism (TRFLP) analysis of human gut microbiota

Author

Li, Fei, Hullar, Meredith A.J., and Lampe, Johanna W.

Subjects

*GENETIC polymorphisms, *METABOLISM, *BIOCHEMISTRY, *ANTHROPOMETRY

Abstract

Abstract: Some compounds originating from the human gut microbial metabolism of exogenous and endogenous substrates may have properties that profoundly affect the host''s physiological processes. The influence of these metabolites on differences in disease risk among individuals could be mediated by metabolism specific to the gut microbial community composition. In this study, we evaluated the effectiveness of terminal restriction fragment polymorphism (TRFLP) as a biomarker of the fecal microbial community (as a surrogate of gut microbiota) for application in human population-based studies. We tested the effects of experimental conditions on DNA quality, DNA quantity, and TRFLP patterns derived from gut bacterial communities. Genomic DNA was extracted from fecal slurries and the bacterial 16S rDNA genes were amplified and analyzed by TRFLP. We found that the composition of the TRFLP fingerprints varied by different extraction procedure. The best quality and quantity of community DNA extracted from fecal material was obtained by using the QIAamp DNA stool minikit (Qiagen, Valencia, CA) with 95 °C incubation and moderate bead beating treatment during the cell-lysis step. Homogenization of fecal samples reduced variation among replicates. Once the TRFLP procedure was optimized, we assessed the methodological and inter-individual variation in gut microbial community fingerprints. The methodological variation ranged from 4.5–8.1% and inter-individual variation was 50.3% for common peaks. In conclusion, standardized TRFLP is a robust, reproducible, and high-throughput method that will provide a useful biomarker for characterizing gut microbiota in human fecal samples. [Copyright &y& Elsevier]

Published

2007