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Development and validation of quantitative PCR assays for HIV-associated cryptococcal meningitis in sub-Saharan Africa: a diagnostic accuracy study

Mbangiwa, T; Sturny-Leclère, A; Lechiile, K; Kajanga, C; Boyer-Chammard, T; Hoving, JC; Leeme, T; Moyo, M; Youssouf, N; Lawrence, DS; et al. Mbangiwa, T; Sturny-Leclère, A; Lechiile, K; Kajanga, C; Boyer-Chammard, T; Hoving, JC; Leeme, T; Moyo, M; Youssouf, N; Lawrence, DS; Mwandumba, H; Mosepele, M; Harrison, TS; Jarvis, JN; Lortholary, O; Alanio, A; Goodall, J; Mawoko, N; Milburn, J; Mmipi, R; Muthoga, C; Ponatshego, P; Rulaganyang, I; Seatla, K; Tlhako, N; Tsholo, K; April, S; Bekiswa, A; Boloko, L; Bookholane, H; Crede, T; Davids, L; Goliath, R; Hlungulu, S; Hoffman, R; Kyepa, H; Masina, N; Maughan, D; Mnguni, T; Moosa, S; Morar, T; Mpalali, M; Naude, J; Oliphant, I; Sayed, S; Sebesho, L; Shey, M; Swanepoel, L; Chasweka, M; Chimang’anga, W; Chimphambano, T; Dziwani, E; Gondwe, E; Kadzilimbile, A; Kateta, S; Kossam, E; Kukacha, C; Lipenga, B; Ndaferankhande, J; Ndalama, M; Shah, R; Singini, A; Stott, K; Zambasa, A; Banda, T; Chikaonda, T; Chitulo, G; Chiwoko, L; Chome, N; Gwin, M; Kachitosi, T; Kamanga, B; Kazembe, M; Kumwenda, E; Kumwenda, M; Maya, C; Mhango, W; Mphande, C; Msumba, L; Munthali, T; Ngoma, D; Nicholas, S; Simwinga, L; Stambuli, A; Tegha, G; Zambezi, J; Ahimbisibwe, C; Akampurira, A; Alice, A; Cresswell, F; Gakuru, J; Kiiza, D; Kisembo, J; Kwizera, R; Kugonza, F; Laker, E; Luggya, T; Lule, A; Musubire, A; Muyise, R; Namujju, O; Ndyetukira, J; Nsangi, L; Okirwoth, M; Sadiq, A; Tadeo, K; Tukundane, A; Williams, D; Atwine, L; Buzaare, P; Collins, M; Emily, N; Inyakuwa, C; Kariisa, S; Mwesigye, J; Niwamanya, S; Rodgers, A; Rukundo, J; Rwomushana, I; Ssemusu, M; Stead, G; Boyd, K; Gondo, S; Kufa, P; Makaha, E; Moyo, C; Mtisi, T; Mudzingwa, S; Mwarumba, T; Zinyandu, T; Dromer, F; Johnstone, P; Hafeez, S (2024) Development and validation of quantitative PCR assays for HIV-associated cryptococcal meningitis in sub-Saharan Africa: a diagnostic accuracy study. The Lancet Microbe, 5 (3). e261-e271. ISSN 2666-5247 https://doi.org/10.1016/s2666-5247(23)00362-2
SGUL Authors: Harrison, Thomas Stephen

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Abstract

Background: HIV-associated cryptococcal meningitis is the second leading cause of AIDS-related deaths, with a 10-week mortality rate of 25–30%. Fungal load assessed by colony-forming unit (CFU) counts is used as a prognostic marker and to monitor response to treatment in research studies. PCR-based assessment of fungal load could be quicker and less labour-intensive. We sought to design, optimise, and validate quantitative PCR (qPCR) assays for the detection, identification, and quantification of Cryptococcus infections in patients with cryptococcal meningitis in sub-Saharan Africa. Methods: We developed and validated species-specific qPCR assays based on DNA amplification of QSP1 (QSP1A specific to Cryptococcus neoformans, QSP1B/C specific to Cryptococcus deneoformans, and QSP1D specific to Cryptococcus gattii species) and a pan-Cryptococcus assay based on a multicopy 28S rRNA gene. This was a longitudinal study that validated the designed assays on cerebrospinal fluid (CSF) of 209 patients with cryptococcal meningitis at baseline (day 0) and during anti-fungal therapy (day 7 and day 14), from the AMBITION-cm trial in Botswana and Malawi (2018–21). Eligible patients were aged 18 years or older and presenting with a first case of cryptococcal meningitis. Findings: When compared with quantitative cryptococcal culture as the reference, the sensitivity of the 28S rRNA was 98·2% (95% CI 95·1–99·5) and of the QSP1 assay was 90·4% (85·2–94·0) in CSF at day 0. Quantification of the fungal load with QSP1 and 28S rRNA qPCR correlated with quantitative cryptococcal culture (R2=0·73 and R2=0·78, respectively). Both Botswana and Malawi had a predominant C neoformans prevalence of 67% (95% CI 55–75) and 68% (57–73), respectively, and lower C gattii rates of 21% (14–31) and 8% (4–14), respectively. We identified ten patients that, after 14 days of treatment, harboured viable but non-culturable yeasts based on QSP1 RNA detection (without any positive CFU in CSF culture). Interpretation: QSP1 and 28S rRNA assays are useful in identifying Cryptococcus species. qPCR results correlate well with baseline quantitative cryptococcal culture and show a similar decline in fungal load during induction therapy. These assays could be a faster alternative to quantitative cryptococcal culture to determine fungal load clearance. The clinical implications of the possible detection of viable but non-culturable cells in CSF during induction therapy remain unclear.

Item Type: Article
Additional Information: Copyright © 2023 The Author(s). Published by Elsevier Ltd. This is an open access article under the CC BY-NC-ND license (http://creativecommons.org/licenses/by-nc-nd/4.0/).
SGUL Research Institute / Research Centre: Academic Structure > Infection and Immunity Research Institute (INII)
Journal or Publication Title: The Lancet Microbe
ISSN: 2666-5247
Language: en
Dates:
DateEvent
15 March 2024Published
8 February 2024Published Online
26 October 2023Accepted
Publisher License: Creative Commons: Attribution-Noncommercial-No Derivative Works 4.0
Projects:
Project IDFunderFunder ID
TRIA2015-1092Wellcome Trusthttp://dx.doi.org/10.13039/100004440
RP-2017-08-ST2-012National Institute for Health and Care Researchhttp://dx.doi.org/10.13039/501100000272
MR/P006922/1Medical Research Councilhttp://dx.doi.org/10.13039/501100000265
URI: https://openaccess.sgul.ac.uk/id/eprint/116224
Publisher's version: https://doi.org/10.1016/s2666-5247(23)00362-2

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