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侵袭性念珠菌属抗真菌药敏试验方法的比较评估以及卡泊芬净中介和耐药菌株中FKS基因突变的检测

Comparative evaluation of antifungal susceptibility testing methods of invasive Candida species and detection of FKS genes mutations in caspofungin intermediate and resistant isolates.

作者信息

ElFeky Dalia Saad, El-Wakil Doaa Mahdy, Mwafy Mai M, Atia Mohamed M A, Gohar Noha Mahmoud

机构信息

Department of Medical Microbiology and Immunology, Faculty of Medicine, Cairo University, Al-Saray Street, Al-Manial, Cairo, 11562, Egypt.

Department of Medical Microbiology and Immunology, Faculty of Medicine, Tanta University, Tanta, Egypt.

出版信息

BMC Infect Dis. 2025 Jan 24;25(1):114. doi: 10.1186/s12879-024-10435-8.

Abstract

BACKGROUND

Fungal invasive infections caused by Candida species pose a substantial public health risk with limited therapeutic options. Antifungal susceptibility testing (AFST) is necessary to optimize the therapy. The study aimed to compare different AFST methods of Candida spp. and detect FKS gene mutations among caspofungin-intermediate and resistant isolates.

METHODS

A total of 60 non-replicative invasive Candida isolates recovered from various clinical samples were included. In-vitro AFST was carried out using the ATB FUNGUS 3, Vitek-2 AST-YS08, and E-test. Hotspot (HS) regions of FKS genes were sequenced for caspofungin-intermediate and resistant isolates.

RESULTS

Candida albicans (58.3%) was the most predominant spp., followed by C. glabrata (28.3%). Based on the clinical breakpoints (CBPs), fluconazole resistance was found in C. albicans (45.7%), C. tropicalis (25%), and the C. parapsilosis isolate, while 35.3% of C. glabrata were susceptible dose-dependent (SDD). None of C. albicans, C. tropicalis, or C. parapsilosis isolates were resistant to voriconazole. Using the epidemiological cut-off values (ECVs) for amphotericin B, 6.7% of isolates were non-wild type (non-WT), including C. guilliermondii (50%), C. tropicalis (25%), and C. glabrata (11.8%), while all C. albicans, C. parapsilosis, and C. kefyr isolates were classified as wild-type (WT). ATB FUNGUS 3 and Vitek-2 had the highest categorical agreement (CA) (83.1%) for amphotericin B, while a lower concordance was detected with voriconazole (23.2%) and fluconazole (52.2%). For caspofungin, Vitek-2 and E-test had a CA of 89.8%. Eleven isolates (10 C. glabrata and one C. parapsilosis) exhibited resistance or intermediate susceptibility to caspofungin (MICs: 0.25‒>32 µg/ml). Molecular characterization of the FKS gene demonstrated that FKS1 mutations V47I, V52K, V56T, D57S, L62F, I71Y, I71Q in the HS1 region, and G7S, P11H mutations in the HS2 region were associated with increased caspofungin MIC values (16 µg/ml). Mutations at the HS1 of the FKS2 gene; K33V, W35K, and W35V; were associated with the highest caspofungin MICs of > 32 µg/ml.

CONCLUSIONS

ATB FUNGUS 3 demonstrated acceptable performance for AFST, however, azole activity against Candida spp. should be interpreted carefully. Novel mutations within HS regions of FKS genes elucidated different levels of caspofungin resistance in C. glabrata and C. parapsilosis isolates.

摘要

背景

念珠菌属引起的真菌侵袭性感染对公众健康构成重大风险,且治疗选择有限。抗真菌药敏试验(AFST)对于优化治疗是必要的。本研究旨在比较念珠菌属不同的AFST方法,并检测卡泊芬净中介及耐药菌株中的FKS基因突变。

方法

共纳入60株从各种临床样本中分离出的非复制性侵袭性念珠菌。使用ATB FUNGUS 3、Vitek-2 AST-YS08和E-test进行体外AFST。对卡泊芬净中介及耐药菌株的FKS基因热点(HS)区域进行测序。

结果

白色念珠菌(58.3%)是最主要的菌种,其次是光滑念珠菌(28.3%)。根据临床断点(CBP),白色念珠菌(45.7%)、热带念珠菌(25%)和近平滑念珠菌分离株中发现氟康唑耐药,而35.3%的光滑念珠菌对氟康唑呈剂量依赖性敏感(SDD)。白色念珠菌、热带念珠菌或近平滑念珠菌分离株对伏立康唑均无耐药。使用两性霉素B的流行病学临界值(ECV),6.7%的分离株为非野生型(非WT),包括季也蒙念珠菌(50%)、热带念珠菌(25%)和光滑念珠菌(11.8%),而所有白色念珠菌、近平滑念珠菌和克菲尔念珠菌分离株均被分类为野生型(WT)。ATB FUNGUS 3和Vitek-2对两性霉素B的分类一致性(CA)最高(83.1%),而与伏立康唑(23.2%)和氟康唑(52.2%)的一致性较低。对于卡泊芬净,Vitek-2和E-test 的CA为89.8%。11株分离株(10株光滑念珠菌和1株近平滑念珠菌)对卡泊芬净表现出耐药或中介敏感性(MIC:0.25‒>32 μg/ml)。FKS基因的分子特征表明,HS1区域的FKS1突变V47I、V52K、V56T、D57S、L62F、I7IY、I71Q以及HS2区域的G7S、P11H突变与卡泊芬净MIC值升高(16 μg/ml)相关。FKS2基因HS1处的突变K33V、W35K和W35V与卡泊芬净MIC>32 μg/ml的最高值相关。

结论

ATB FUNGUS 3在AFST中表现出可接受的性能,然而,唑类对念珠菌属的活性应谨慎解释。FKS基因HS区域内的新突变阐明了光滑念珠菌和近平滑念珠菌分离株中不同水平的卡泊芬净耐药性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f4ef/11760087/2367629e2f12/12879_2024_10435_Fig1_HTML.jpg

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