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CAMP阴性菌株表现出编码CAMP因子的基因的全部或部分染色体缺失。

CAMP-negative strains exhibited complete or partial chromosomal deletions of the CAMP-factor encoding gene .

作者信息

Lai Xixi, Chen Meihong, Wang Jianwei, Wang Junjun, Lv Hui, Xie Haihua, He Wenjuan, Chen Dongjie, Huang Yi, Cai Pengwei, Zheng Lilan

机构信息

Department of Clinical Laboratory, Fujian Provincial Hospital, Fuzhou University Affiliated Provincial Hospital, Fuzhou, China.

Shengli Clinical Medical College, Fujian Medical University, Fuzhou, China.

出版信息

Microbiol Spectr. 2025 Apr 9;13(5):e0325724. doi: 10.1128/spectrum.03257-24.

Abstract

UNLABELLED

Universal antepartum group B streptococcus (GBS) screening and intrapartum antibiotic prophylaxis (IAP) have effectively reduced early-onset GBS infections. However, GBS strains with chromosomal deletions affecting the gene may produce false negatives in both the CAMP test and -based molecular diagnostics, potentially increasing the risk of neonatal infections. Vaginal swabs were collected from pregnant women at 35-37 weeks of gestation in our hospital and cultured on agar. Suspected GBS strains were initially identified using the CAMP test and then confirmed with the VITEK-2 system. CAMP-negative GBS strains underwent additional testing by qPCR, 16S rDNA, serotyping, and multilocus sequence typing (MLST). PCR for the gene and whole-genome sequencing were performed on CAMP-negative strains. From 5,794 samples, 526 (9.1%) GBS strains, including 19 (3.6%) CAMP-negative strains and 2 strains from the same patient, were isolated. All 19 CAMP-negative strains were serotypes III and ST862. Among these strains, only one strain was positive by qPCR, whereas all tested positive with a multitarget qPCR kit for and . PCR amplification upstream of the gene produced a specific band in strain PP669713 only, suggesting N-terminal gene retention in PP669713 and complete loss in the other strains. Whole-genome sequencing confirmed a chromosomal deletion in PP669713. Antibiotic susceptibility testing revealed no resistance to penicillin. However, CAMP-positive strains presented a greater prevalence of resistance to ciprofloxacin, and levofloxacin than CAMP-negative strains did. Our study highlights the potential risk of missed GBS detection using CAMP tests and -targeted molecular assays.

IMPORTANCE

Our work makes several novel contributions to the field. (i) We report the first documented case of a C-terminal deletion of the gene in a CAMP-negative GBS strain, demonstrating that both N-terminal and C-terminal regions are essential for cohemolytic activity. (ii) Our findings reveal that CAMP-negative GBS strains (3.6% of isolates) are more prevalent than previously recognized, with most cases resulting from complete chromosomal deletions of the gene. (iii) We provide evidence that single-target molecular assays targeting only the gene may miss GBS detection, highlighting the necessity for multi-target approaches in clinical diagnostics. (iv) We demonstrate a unique antibiotic resistance pattern in CAMP-negative strains, showing significantly lower resistance to certain antibiotics compared to CAMP-positive strains.

摘要

未标注

普遍的产前B族链球菌(GBS)筛查和产时抗生素预防(IAP)已有效降低早发性GBS感染。然而,影响该基因的染色体缺失的GBS菌株可能在CAMP试验和基于该基因的分子诊断中产生假阴性,从而可能增加新生儿感染的风险。在我院对妊娠35 - 37周的孕妇采集阴道拭子并在琼脂上培养。疑似GBS菌株最初通过CAMP试验鉴定,然后用VITEK - 2系统确认。CAMP阴性的GBS菌株通过qPCR、16S rDNA、血清分型和多位点序列分型(MLST)进行额外检测。对CAMP阴性菌株进行该基因的PCR和全基因组测序。从5794份样本中分离出526株(9.1%)GBS菌株,包括19株(3.6%)CAMP阴性菌株以及来自同一患者的2株。所有19株CAMP阴性菌株均为血清型III和ST862。在这些菌株中,仅1株通过qPCR检测该基因呈阳性,而所有菌株使用针对该基因和另一基因的多靶点qPCR试剂盒检测均呈阳性。该基因上游的PCR扩增仅在菌株PP669713中产生一条特异性条带,表明PP669713中该基因N端保留而其他菌株中该基因完全缺失。全基因组测序证实PP669713存在染色体缺失。抗生素敏感性试验显示对青霉素无耐药性。然而,CAMP阳性菌株对环丙沙星和左氧氟沙星的耐药率高于CAMP阴性菌株。我们的研究强调了使用CAMP试验和针对该基因的分子检测方法漏检GBS的潜在风险。

重要性

我们的工作为该领域做出了多项新贡献。(i)我们报告了首例记录在案的CAMP阴性GBS菌株中该基因C端缺失的病例,证明N端和C端区域对协同溶血活性均至关重要。(ii)我们的研究结果表明,CAMP阴性GBS菌株(占分离株的3.6%)比之前认识到的更为普遍,大多数病例是由于该基因的染色体完全缺失。(iii)我们提供证据表明仅针对该基因的单靶点分子检测可能漏检GBS,突出了临床诊断中采用多靶点方法的必要性。(iv)我们展示了CAMP阴性菌株独特的抗生素耐药模式,显示与CAMP阳性菌株相比,对某些抗生素的耐药性显著更低。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3551/12054153/b5f0a8e6efa2/spectrum.03257-24.f001.jpg

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