Detection of Rickettsia rickettsii, Rickettsia parkeri, and Rickettsia akari in Skin Biopsy Specimens Using a Multiplex Real-time Polymerase Chain Reaction Assay

Denison, Amy M.; Amin, Bijal D.; Nicholson, William L.; Paddock, Christopher D.

doi:10.1093/cid/ciu358

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CDC STACKS serves as an archival repository of CDC-published products including scientific findings, journal articles, guidelines, recommendations, or other public health information authored or co-authored by CDC or funded partners. As a repository, CDC STACKS retains documents in their original published format to ensure public access to scientific information.

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Detection of Rickettsia rickettsii, Rickettsia parkeri, and Rickettsia akari in Skin Biopsy Specimens Using a Multiplex Real-time Polymerase Chain Reaction Assay

9 1 2014
By Denison, Amy M. ; Amin, Bijal D. ; Nicholson, William L. ; ...
http://dx.doi.org/10.1093/cid/ciu358
Source: Clin Infect Dis. 59(5):635-642

English

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Details:

Alternative Title:

Clin Infect Dis
Personal Author:

Denison, Amy M. ; Amin, Bijal D. ; Nicholson, William L. ; Paddock, Christopher D.

Denison, Amy M. ; Amin, Bijal D. ; Nicholson, William L. ; Paddock, Christopher D. Less -
Description:

Background

Rickettsia rickettsii, Rickettsia parkeri, and Rickettsia akari are the most common causes of spotted fever group rickettsioses indigenous to the United States. Infected patients characteristically present with a maculopapular rash, often accompanied by an inoculation eschar. Skin biopsy specimens are often obtained from these lesions for diagnostic evaluation. However, a species-specific diagnosis is achieved infrequently from pathologic specimens because immunohistochemical stains do not differentiate among the causative agents of spotted fever group rickettsiae, and existing polymerase chain reaction (PCR) assays generally target large gene segments that may be difficult or impossible to obtain from formalin-fixed tissues.

Methods

This work describes the development and evaluation of a multiplex real-time PCR assay for the detection of these 3 Rickettsia species from formalin-fixed, paraffin-embedded (FFPE) skin biopsy specimens.

Results

The multiplex PCR assay was specific at discriminating each species from FFPE controls of unrelated bacterial, viral, protozoan, and fungal pathogens that cause skin lesions, as well as other closely related spotted fever group Rickettsia species.

Conclusions

This multiplex real-time PCR demonstrates greater sensitivity than nested PCR assays in FFPE tissues and provides an effective method to specifically identify cases of Rocky Mountain spotted fever, rickettsialpox, and R. parkeri rickettsiosis by using skin biopsy specimens.
Subjects:

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Article Biopsy Citrate (si)-Synthase Exanthema Humans Real-time PCR Real-Time Polymerase Chain Reaction Rickettsia Rickettsia Akari Rickettsia Infections Rickettsia Rickettsii Rocky Mountain Spotted Fever Sensitivity And Specificity Skin Skin Biopsies
Source:

Clin Infect Dis. 59(5):635-642
Pubmed ID:

24829214
Pubmed Central ID:

PMC4568984
Document Type:

Journal Article
Funding:

CC999999/Intramural CDC HHSUnited States/
Volume:

59
Issue:

5
Collection(s):

CDC Public Access
Main Document Checksum:

[+]

urn:sha256:030267c6ccd41cfd6674f1a29526edde5336a984fe8fe74eaabf1c350d212e50
Download URL:

https://stacks.cdc.gov/view/cdc/34289/cdc_34289_DS1.pdf
File Type:

[PDF-1007.59 KB]

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