Rapid DNA fingerprinting of pathogens by flow cytometry

Larson, Erica J.; Hakovirta, Janetta R.; Cai, Hong; Jett, James H.; Burde, Stefan; Keller, Richard A.; Marrone, Babetta L.

doi:10.1002/1097-0320(20001101)41:3<203::aid-cyto7>3.0.co;2-2

Cited by 22 publications

(23 citation statements)

References 30 publications

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“…Staphylococcus aureus Mu50 (#700699; ATCC, Manassas, VA) DNA was extracted from agarose plugs according to previously described procedures (28). Briefly, overnight cultures were used to prepare 1.5% low-melting agarose (InCert; FMC BioProducts, Rockland, ME) plugs, each containing ϳ10 7 cells.…”

Section: Materials and Methods Sample Preparationmentioning

confidence: 99%

“…Note that the fingerprints shown in Figure 8 have been normalized or offset to facilitate direct comparison. While the data used to produce the histogram in Figure 8b represents only 4% of the entire data set, the prominent, identifying features used from FCM data sets to discriminate bacteria at the species and strain level are all present (28,42). Thus, bacterial discrimination by FCM, previously demonstrated with large data sets, is feasible based on the analysis of as few as 10 genomes.…”

Section: Application To Flow Cytometry Sizing Of Dna Fragmentsmentioning

confidence: 95%

“…Bacterial DNA fingerprinting represents a significantly more difficult task, relative to viral fingerprinting, due to the increased number of fragment species as well as the fact that many fragments are larger and are therefore more fragile. Nevertheless, our group has demonstrated bacterial discrimination at the species and strain level based on FCM results with fragments Յ400 kb (28,42,43).…”

Section: Application To Flow Cytometry Sizing Of Dna Fragmentsmentioning

confidence: 97%

“…The data used to create this histogram was collected over several minutes and corresponds to ϳ600 digested Mu50 genomes. This sample corresponds to approximately 10 3 times less DNA than would be required for PFGE analysis (28,42,43). A conservative estimate of N min for this sample is N ϭ 10 which corresponds to the analysis of only 10 digested bacterial genomes.…”

Section: Application To Flow Cytometry Sizing Of Dna Fragmentsmentioning

confidence: 99%

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Statistics of single‐molecule measurements: Applications in flow‐cytometry sizing of DNA fragments

Ferris¹,

Habbersett²,

Wolinsky³

et al. 2004

Cytometry Pt A

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Background:The measurement of physical properties from single molecules has been demonstrated. However, the majority of single-molecule studies report values based on relatively large data sets (e.g., N Ͼ 50). While there are studies that report physical quantities based on small sample sets, there has not been a detailed statistical analysis relating sample size to the reliability of derived parameters. Methods: Monte Carlo simulations and multinomial analysis, dependent on quantifiable experimental parameters, were used to determine the minimum number of singlemolecule measurements required to produce an accurate estimate of a population mean. Simulation results were applied to the fluorescence-based sizing of DNA fragments by ultrasensitive flow cytometry (FCM). Results: Our simulations show, for an analytical technique with a 10% CV, that the average of as few as five

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Section: Materials and Methods Sample Preparationmentioning

confidence: 99%

Section: Application To Flow Cytometry Sizing Of Dna Fragmentsmentioning

confidence: 95%

Section: Application To Flow Cytometry Sizing Of Dna Fragmentsmentioning

confidence: 97%

Section: Application To Flow Cytometry Sizing Of Dna Fragmentsmentioning

confidence: 99%

See 2 more Smart Citations

Statistics of single‐molecule measurements: Applications in flow‐cytometry sizing of DNA fragments

Ferris¹,

Habbersett²,

Wolinsky³

et al. 2004

Cytometry Pt A

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“…For instance, PFGE requires relatively large quantities of DNA (Ն200 ng of DNA or ϳ10 7 bacterial cells [33] or at least 1 ng of DNA per band [42]). Typically, bacterial samples must be cultured to obtain this amount of DNA (culturing can require up to 48 h and some bacteria cannot be cultured).…”

mentioning

confidence: 99%

Performance Assessment of DNA Fragment Sizing by High-Sensitivity Flow Cytometry and Pulsed-Field Gel Electrophoresis

et al. 2004

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The sizing of restriction fragments is the chief analytical technique utilized in the production of DNA fingerprints. Few techniques have been able to compete with pulsed-field gel electrophoresis (PFGE), which is capable of discriminating among bacteria at species and strain levels by resolving restriction fragments. However, an ultrasensitive flow cytometer (FCM) developed in our lab has also demonstrated the ability to discriminate bacteria at species and strain levels. The abilities of FCM warrant a quantitative parallel comparison with PFGE to assess and evaluate the accuracy and precision of DNA fragment sizing by both techniques. Replicate samples of Staphylococcus aureus Mu50 were analyzed along with two clinical S. aureus isolates. The absolute fragment sizing accuracy was determined for PFGE (5% ؎ 2%) and FCM (4% ؎ 4%), with sequence-predicted Mu50 SmaI fragment sizes used as a reference. Precision was determined by simple arithmetic methods (relative standard deviation for PFGE [RSD PFGE ] ‫؍‬ 3% ؎ 2% and RSD FCM ‫؍‬ 1.2% ؎ 0.8%) as well as by the use of dendrograms derived from Dice coefficient-unweighted pair group method with arithmetic averages (UPGMA) and Pearson-UPGMA analyses. All quantitative measures of PFGE and FCM precision were equivalent, within error. The precision of both methods was not limited by any single sample preparation or analysis step that was tracked in this study. Additionally, we determined that the curve-based clustering of fingerprint data provided a more informative and useful assessment than did traditional bandbased methods.DNA fragment sizing is arguably the most widely used analytical method in molecular biology, biochemistry, and microbiology. Specific applications of DNA fragment sizing include microbe identification and discrimination, genotyping, and sequencing. Traditionally, DNA fragments are characterized via size-dependent separation methods such as gel electrophoresis.Conventional gel electrophoresis, using a solid polymer (e.g., agarose or polyacrylamide) and a static electric field, is ubiquitous in today's molecular biology and biochemistry labs. Such methods are routinely used to separate and size DNA fragments of Յ20 kb (4).Pulsed-field gel electrophoresis (PFGE), developed in 1984 by Schwartz et al. (44), extended the fragment sizing range to over 1 Mb (4,6,9,19,44). For PFGE, large DNA fragments (i.e., Ͼ10 kb) are separated in an agarose gel by a pulsed electric field. A popular application of PFGE has been strainlevel bacterial fingerprinting through the sizing of DNA fragments resulting from the digestion of whole genomic DNAs with rare-cutting restriction endonucleases (5,11,28,35,47,49). Macrorestriction-based bacterial fingerprinting has found applications primarily in the public health and food safety industries. For example, the Centers for Disease Control and Prevention (CDC) have formed PulseNet, the National Molecular Subtyping Network for Foodborne Disease Surveillance (46; http://www.cdc.gov/pulsenet). PulseNet utilizes macrorestriction fi...

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