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High Applicability of a Novel Method for gp60-Based Subtyping of Cryptosporidium meleagridis

机译:基于gp60的隐孢子虫亚型新方法的高度适用性

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摘要

Cryptosporidium meleagridis is a common cause of cryptosporidiosis in avian hosts and the third most common species involved in human cryptosporidiosis. Sequencing of the highly polymorphic 60-kDa glycoprotein (gp60) gene is a frequently used tool for investigation of the genetic diversity and transmission dynamics of Cryptosporidium. However, few studies have included gp60 sequencing of C. meleagridis. One explanation may be that the gp60 primers currently in use are based on Cryptosporidium hominis and Cryptosporidium parvum sequence data, potentially limiting successful amplification of the C. meleagridis gp60 gene. We therefore aimed to design primers for better gp60 subtyping of C. meleagridis. Initially, ∼1,440 bp of the gp60 locus of seven C. meleagridis isolates were amplified using primers flanking the open reading frame. The obtained sequence data (∼1,250 bp) were used to design primers for a nested PCR targeting C. meleagridis. Twenty isolates (16 from human and 4 from poultry) previously identified as C. meleagridis by analysis of small subunit (SSU) rRNA genes were investigated. Amplicons of the expected size (∼900 bp) were obtained from all 20 isolates. The subsequent sequence analysis identified 3 subtype families and 10 different subtypes. The most common subtype family, IIIb, was identified in 12 isolates, represented by 6 subtypes, 4 new and 2 previously reported. Subtype family IIIe was found in 3 isolates represented by 3 novel, distinct subtypes. Finally, IIIgA31G3R1 was found in 1 human isolate and 4 poultry isolates, all originating from a previously reported C. meleagridis outbreak at a Swedish organic farm.
机译:隐孢子虫是禽寄主中隐孢子虫病的常见原因,也是人类隐孢子虫病的第三大常见物种。高度多态的60 kDa糖蛋白(gp60)基因的测序是研究隐孢子虫的遗传多样性和传播动力学的常用工具。但是,很少有研究包括梅氏梭菌的gp60测序。一种解释可能是,当前使用的gp60引物基于人隐孢子虫和小隐孢子虫序列数据,可能会限制meleagridis C. gp60基因的成功扩增。因此,我们的目的是设计引物,以更好地对肉毒梭菌进行gp60亚型分析。最初,使用侧翼于开放阅读框的引物,扩增了七个麻省分枝杆菌的gp60基因座的约1,440 bp。获得的序列数据(〜1,250 bp)被用于设计针对meleagridis的巢式PCR的引物。通过分析小亚基(SSU)rRNA基因,鉴定了二十种分离株(人中有16种,家禽中有4种),以前被鉴定为肉食梭状芽胞杆菌。从所有20个分离株中均获得了预期大小的扩增子(约900 bp)。随后的序列分析确定了3个亚型家族和10个不同的亚型。在12种分离物中鉴定出最常见的亚型家族,即IIIb,由6种亚型,4种新亚型和2种先前报道的亚型代表。在3种新的,独特的亚型代表的3种分离物中发现了IIIe家族。最后,在1个人类分离株和4个家禽分离株中发现了IIIgA31G3R1,这些分离株均来自先前报道的瑞典有机农场的C. meleagridis暴发。

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