1Amsterdam UMC, University of Amsterdam, Medical Microbiology, Amsterdam, The Netherlands.
2Amsterdam UMC, University of Amsterdam, Clinical Genetics, Core Facility Genomics, Amsterdam, The Netherlands.
Antimicrob Resist Infect Control. 2019 Sep 23;8:153. doi: 10.1186/s13756-019-0604-5. eCollection 2019.
Recognition of nosocomial outbreaks with antimicrobial resistant (AMR) pathogens and appropriate infection prevention measures are essential to limit the consequences of AMR pathogens to patients in hospitals. Because unrelated, but genetically similar AMR pathogens may circulate simultaneously, rapid high-resolution molecular typing methods are needed for outbreak management. We compared amplified fragment length polymorphism (AFLP) and whole genome sequencing (WGS) during a nosocomial outbreak of vancomycin-resistant (VRE) that spanned 5 months.
Hierarchical clustering of AFLP profiles was performed using unweighted pair-grouping and similarity coefficients were calculated with Pearson correlation. For WGS-analysis, core single nucleotide polymorphisms (SNPs) were used to calculate the pairwise distance between isolates, construct a maximum likelihood phylogeny and establish a cut-off for relatedness of epidemiologically linked VRE isolates. SNP-variations in the gene cluster were compared to increase the comparative resolution. Technical replicates of 2 isolates were sequenced to determine the number of core-SNPs derived from random sequencing errors.
Of the 721 patients screened for VRE carriage, AFLP assigned isolates of 22 patients to the outbreak cluster. According to WGS, all 22 isolates belonged to ST117 but only 21 grouped in a tight phylogenetic cluster and carried resistance gene clusters. Sequencing of technical replicates showed that 4-5 core-SNPs were derived by random sequencing errors. The cut-off for relatedness of epidemiologically linked VRE isolates was established at ≤7 core-SNPs. The discrepant isolate was separated from the index isolate by 61 core-SNPs and the gene cluster was absent. In AFLP analysis this discrepant isolate was indistinguishable from the other outbreak isolates, forming a cluster with 92% similarity (cut-off for identical isolates ≥90%). The inclusion of the discrepant isolate in the outbreak resulted in the screening of 250 patients and quarantining of an entire ward.
AFLP was a rapid and affordable screening tool for characterising hospital VRE outbreaks. For in-depth understanding of the outbreak WGS was needed. Compared to AFLP, WGS provided higher resolution typing of VRE isolates with implications for outbreak management.
识别医院内耐抗生素(AMR)病原体的爆发和采取适当的感染预防措施对于限制 AMR 病原体对医院患者的影响至关重要。由于不相关但遗传上相似的 AMR 病原体可能同时传播,因此需要快速、高分辨率的分子分型方法进行爆发管理。我们比较了在跨越 5 个月的万古霉素耐药(VRE)医院爆发期间进行的扩增片段长度多态性(AFLP)和全基因组测序(WGS)。
使用非加权对群组聚类分析 AFLP 图谱,并使用皮尔逊相关系数计算相似性系数。对于 WGS 分析,使用核心单核苷酸多态性(SNP)计算分离株之间的成对距离,构建最大似然系统发育,并建立与流行病学相关的 VRE 分离株的亲缘关系的截止值。比较基因簇中的 SNP 变异以提高比较分辨率。对 2 个分离株的技术重复进行测序,以确定源自随机测序错误的核心 SNP 的数量。
在对 721 名 VRE 携带者进行筛查的患者中,AFLP 将 22 名患者的分离株分配到爆发群中。根据 WGS,所有 22 个分离株均属于 ST117,但只有 21 个分离株紧密聚类并携带耐药基因簇。技术重复的测序表明,4-5 个核心 SNP 是由随机测序错误引起的。将流行病学相关 VRE 分离株的亲缘关系截止值设定为≤7 个核心 SNP。分离株与索引分离株相差 61 个核心 SNP,且基因簇缺失。在 AFLP 分析中,该分离株与其他爆发分离株无法区分,形成了一个相似度为 92%(相似度为 90%以上的相同分离株的截止值)的聚类。将差异分离株纳入爆发会导致对 250 名患者进行筛查,并隔离整个病房。
AFLP 是一种快速且经济实惠的方法,用于表征医院内 VRE 爆发。为了深入了解爆发情况,需要进行 WGS。与 AFLP 相比,WGS 为 VRE 分离株提供了更高分辨率的分型,这对爆发管理具有重要意义。
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