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Orthopoxvirus Testing Challenges for Persons in Populations at Low Risk or Without Known Epidemiologic Link to Monkeypox - United States, 2022

Overview
Journal MMWR Morb Mortal Wkly Rep
Date 2022 Sep 8
PMID 36074752
Authors
Faisal S Minhaj
Julia K Petras
Jennifer A Brown
Anil T Mangla
Kelly Russo
Christina Willut
Michelle Lee
Jason Beverley
Rachel Harold
Lauren Milroy
Brian Pope
Emily Gould
Cole Beeler
Jack Schneider
Heba H Mostafa
Shana Godfred-Cato
Eleanor S Click
Brian F Borah
Romeo R Galang
Shama Cash-Goldwasser
Joshua M Wong
David W McCormick
Patricia A Yu
Victoria Shelus
Ann Carpenter
Sabrina Schatzman
David Lowe
Michael B Townsend
Whitni Davidson
Nhien T Wynn
Panayampalli S Satheshkumar
Siobhan M OConnor
Kevin OLaughlin
Agam K Rao
Andrea M McCollum
Maria E Negron
Christina L Hutson
Johanna S Salzer
Affiliations
Soon will be listed here.
Abstract

Since May 2022, approximately 20,000 cases of monkeypox have been identified in the United States, part of a global outbreak occurring in approximately 90 countries and currently affecting primarily gay, bisexual, and other men who have sex with men (MSM) (1). Monkeypox virus (MPXV) spreads from person to person through close, prolonged contact; a small number of cases have occurred in populations who are not MSM (e.g., women and children), and testing is recommended for persons who meet the suspected case definition* (1). CDC previously developed five real-time polymerase chain reaction (PCR) assays for detection of orthopoxviruses from lesion specimens (2,3). CDC was granted 510(k) clearance for the nonvariola-orthopoxvirus (NVO)-specific PCR assay by the Food and Drug Administration. This assay was implemented within the Laboratory Response Network (LRN) in the early 2000s and became critical for early detection of MPXV and implementation of public health action in previous travel-associated cases as well as during the current outbreak (4-7). PCR assays (NVO and other Orthopoxvirus laboratory developed tests [LDT]) represent the primary tool for monkeypox diagnosis. These tests are highly sensitive, and cross-contamination from other MPXV specimens being processed, tested, or both alongside negative specimens can occasionally lead to false-positive results. This report describes three patients who had atypical rashes and no epidemiologic link to a monkeypox case or known risk factors; these persons received diagnoses of monkeypox based on late cycle threshold (Ct) values ≥34, which were false-positive test results. The initial diagnoses were followed by administration of antiviral treatment (i.e., tecovirimat) and JYNNEOS vaccine postexposure prophylaxis (PEP) to patients' close contacts. After receiving subsequent testing, none of the three patients was confirmed to have monkeypox. Knowledge gained from these and other cases resulted in changes to CDC guidance. When testing for monkeypox in specimens from patients without an epidemiologic link or risk factors or who do not meet clinical criteria (or where these are unknown), laboratory scientists should reextract and retest specimens with late Ct values (based on this report, Ct ≥34 is recommended) (8). CDC can be consulted for complex cases including those that appear atypical or questionable cases and can perform additional viral species- and clade-specific PCR testing and antiorthopoxvirus serologic testing.

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Paediatric, maternal, and congenital mpox: a systematic review and meta-analysis.

Clemente N, Coles C, Paixao E, Brickley E, Whittaker E, Alfven T Lancet Glob Health. 2024; 12(4):e572-e588.

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Repeat testing of mpox specimens with late CTs improves detection of potential false positive cases.

Shean R, Hymas W, Klein J, Pyne M, Hillyard D, Bradley B J Clin Microbiol. 2024; 62(2):e0127523.

PMID: 38193685 PMC: 10865812. DOI: 10.1128/jcm.01275-23.

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