Detection and identification of mycobacteria in fixed stained smears and formalin‐fixed paraffin‐embedded tissues using PCR. (26th October 2013)
- Record Type:
- Journal Article
- Title:
- Detection and identification of mycobacteria in fixed stained smears and formalin‐fixed paraffin‐embedded tissues using PCR. (26th October 2013)
- Main Title:
- Detection and identification of mycobacteria in fixed stained smears and formalin‐fixed paraffin‐embedded tissues using PCR
- Authors:
- Reppas, G.
Fyfe, J.
Foster, S.
Smits, B.
Martin, P.
Jardine, J.
Lam, A.
O'Brien, C.
Malik, R. - Abstract:
- <abstract abstract-type="main" id="jsap12149-abs-0001"> <title> <x xml:space="preserve">Abstract</x> </title> <sec id="jsap12149-sec-0001" sec-type="section"> <title>Objective</title> <p id="jsap12149-para-0001"> <bold>To determine the feasibility of using polymerase chain reaction to amplify DNA from methanol‐fixed, Romanowsky‐stained and Ziehl‐Neelsen‐stained smears to confirm the presence of mycobacteria.</bold> </p> </sec> <sec id="jsap12149-sec-0002" sec-type="section"> <title>Materials and Methods</title> <p id="jsap12149-para-0002"> <bold>Tissue was obtained from 10 archival slides and 27 slides from a prospective series of consecutive cases. Phosphate buffered saline (500 μL) was pipetted onto a stained smear (on a glass slide) using a disposable filtered pipette tip. The material adherent to the slide was scraped from its surface and drawn up into the saline. Routine DNA extraction and purification was carried out before nested polymerase chain reaction testing targeting the 16S‐23S internal transcribed spacer region or a TaqMan real‐time polymerase chain reaction. The real‐time polymerase chain reaction was also used on thick sections cut from formalin‐fixed paraffin‐embedded tissue blocks from 24 canine leproid granulomas.</bold> </p> </sec> <sec id="jsap12149-sec-0003" sec-type="section"> <title>Results</title> <p id="jsap12149-para-0003"> <bold>Mycobacterial DNA was detected in 34 of 37 slides. Polymerase chain reaction products could not be amplified from three<abstract abstract-type="main" id="jsap12149-abs-0001"> <title> <x xml:space="preserve">Abstract</x> </title> <sec id="jsap12149-sec-0001" sec-type="section"> <title>Objective</title> <p id="jsap12149-para-0001"> <bold>To determine the feasibility of using polymerase chain reaction to amplify DNA from methanol‐fixed, Romanowsky‐stained and Ziehl‐Neelsen‐stained smears to confirm the presence of mycobacteria.</bold> </p> </sec> <sec id="jsap12149-sec-0002" sec-type="section"> <title>Materials and Methods</title> <p id="jsap12149-para-0002"> <bold>Tissue was obtained from 10 archival slides and 27 slides from a prospective series of consecutive cases. Phosphate buffered saline (500 μL) was pipetted onto a stained smear (on a glass slide) using a disposable filtered pipette tip. The material adherent to the slide was scraped from its surface and drawn up into the saline. Routine DNA extraction and purification was carried out before nested polymerase chain reaction testing targeting the 16S‐23S internal transcribed spacer region or a TaqMan real‐time polymerase chain reaction. The real‐time polymerase chain reaction was also used on thick sections cut from formalin‐fixed paraffin‐embedded tissue blocks from 24 canine leproid granulomas.</bold> </p> </sec> <sec id="jsap12149-sec-0003" sec-type="section"> <title>Results</title> <p id="jsap12149-para-0003"> <bold>Mycobacterial DNA was detected in 34 of 37 slides. Polymerase chain reaction products could not be amplified from three archived smears stained using the Ziehl‐Neelsen acid‐fast method, probably because its harsher fixation damaged the DNA. With the nested polymerase chain reaction, species identification using internal transcribed spacer sequence analysis was achieved in all instances, diagnosing a wide range of mycobacteria. The real‐time polymerase chain reaction detected <italic>Mycobacterium</italic> sp. <italic>CLG</italic> DNA within all 24 formalin‐fixed paraffin‐embedded specimens tested.</bold> </p> </sec> <sec id="jsap12149-sec-0004" sec-type="section"> <title>Clinical Significance</title> <p id="jsap12149-para-0004"> <bold>This technique should provide a non‐invasive and cost‐effective means of diagnosing mycobacterial infections.</bold> </p> </sec> </abstract> … (more)
- Is Part Of:
- Journal of small animal practice. Volume 54:Number 12(2013:Dec.)
- Journal:
- Journal of small animal practice
- Issue:
- Volume 54:Number 12(2013:Dec.)
- Issue Display:
- Volume 54, Issue 12 (2013)
- Year:
- 2013
- Volume:
- 54
- Issue:
- 12
- Issue Sort Value:
- 2013-0054-0012-0000
- Page Start:
- 638
- Page End:
- 646
- Publication Date:
- 2013-10-26
- Subjects:
- Veterinary medicine -- Periodicals
Veterinary Medicine -- Periodicals
636.089 - Journal URLs:
- http://onlinelibrary.wiley.com/journal/10.1111/(ISSN)1748-5827 ↗
http://www.blackwell-synergy.com/loi/jsap ↗
http://www.ingentaconnect.com/content/0022-4510 ↗
http://www.ingentaconnect.com/content/bva/jsap ↗
http://onlinelibrary.wiley.com/ ↗ - DOI:
- 10.1111/jsap.12149 ↗
- Languages:
- English
- ISSNs:
- 0022-4510
- Deposit Type:
- Legaldeposit
- View Content:
- Available online (eLD content is only available in our Reading Rooms) ↗
- Physical Locations:
- British Library DSC - 5064.700000
British Library DSC - BLDSS-3PM
British Library STI - ELD Digital store - Ingest File:
- 2959.xml