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Early diagnosis and monitoring of mucormycosis by detection of circulating DNA in serum: retrospective analysis of 44 cases collected through the French Surveillance Network of Invasive Fungal Infections (RESSIF)

Male 0301 basic medicine [SDV]Life Sciences [q-bio] 610 Comorbidity 630 Quantitative PCR 03 medical and health sciences [SDV.MHEP.MI]Life Sciences [q-bio]/Human health and pathology/Infectious diseases Diagnosis Humans Mucormycosis DNA, Fungal [SDV.MP.MYC]Life Sciences [q-bio]/Microbiology and Parasitology/Mycology Aged Retrospective Studies Aged, 80 and over Middle Aged [SDV.MP.MYC] Life Sciences [q-bio]/Microbiology and Parasitology/Mycology Survival Analysis 3. Good health [SDV] Life Sciences [q-bio] monitoring Population Surveillance [SDV.MHEP.MI] Life Sciences [q-bio]/Human health and pathology/Infectious diseases Mucorales Female France Fungemia
DOI: 10.1016/j.cmi.2015.12.006 Publication Date: 2015-12-18T00:33:54Z
Abstract Supplemental Material References Cited by
AUTHORS (51)
L. Millon
R. Herbrecht
F. Grenouillet
F. Morio
A. Alanio
V. Letscher-Bru
S. Cassaing
T. Chouaki
C. Kauffmann-Lacroix
P. Poirier
D. Toubas
O. Augereau
S. Rocchi
D. Garcia-Hermoso
S. Bretagne
H. Dupont
J.P. Marolleau
A. Totet
C. Damiani
A. Berceanu
F. Larosa
J. Bonhomme
C. Chabrot
B. Bouteille
D. Boutoille
T. Gastinne
P. Peterlin
M. Gari Toussaint
D. Poisson
D. Briet
J. Buret
M. Legrand
B. Denis
E. Raffoux
A. Bergeron
A. Veinstein
C. Godet
Y. N'guyen
S. Diallo
M. Sabou
J. Denis
M.P. Ledoux
C. Recher
J. Ruiz
G. Desoubeaux
E. Bailly
E. Chachaty
F. Dromer
O. Lortholary
K. Sitbon
D. Hoinard
ABSTRACT
The main objective of this study was to assess the diagnostic performance of a set of three Mucorales quantitative PCR assays in a retrospective multicentre study. Mucormycosis cases were recorded thanks to the French prospective surveillance programme (RESSIF network). The day of sampling of the first histological or mycological positive specimen was defined as day 0 (D0). Detection of circulating DNA was performed on frozen serum samples collected from D-30 to D30, using quantitative PCR assays targeting Rhizomucor, Lichtheimia, Mucor/Rhizopus. Forty-four patients diagnosed with probable (n = 19) or proven (n = 25) mucormycosis were included. Thirty-six of the 44 patients (81%) had at least one PCR-positive serum. The first PCR-positive sample was observed 9 days (range 0-28 days) before diagnosis was made using mycological criteria and at least 2 days (range 0-24 days) before imaging. The identifications provided with the quantitative PCR assays were all concordant with culture and/or PCR-based identification of the causal species. Survival rate at D84 was significantly higher for patients with an initially positive PCR that became negative after treatment initiation than for patients whose PCR remained positive (48% and 4%, respectively; p <10-6). The median time for complete negativity of PCR was 7 days (range 3-19 days) after initiation of l-AmB treatment. Despite some limitations due to the retrospective design of the study, we showed that Mucorales quantitative PCR could not only confirm the mucormycosis diagnosis when other mycological arguments were present but could also anticipate this diagnosis. Quantification of DNA loads may also be a useful adjunct to treatment monitoring.
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