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通过反向线印迹法同时检测和区分感染小反刍动物的泰勒虫和巴贝斯虫寄生虫

Simultaneous detection and differentiation of Theileria and Babesia parasites infecting small ruminants by reverse line blotting.

作者信息

Schnittger Leonhard, Yin Hong, Qi Bai, Gubbels Marc J, Beyer Doreen, Niemann Stefan, Jongejan Frans, Ahmed Jabbar S

机构信息

Department of Immunology and Cell Biology, Research Centre Borstel, Parkallee 22, 23845 Borstel, Germany.

出版信息

Parasitol Res. 2004 Feb;92(3):189-96. doi: 10.1007/s00436-003-0980-9. Epub 2003 Dec 3.

Abstract

Characteristic sequence signatures were identified within the hypervariable region 4 (V4 region) of the small ribosomal RNA gene of ovine/caprine piroplasm species including Theileria lestoquardi, T. ovis, T. separata, Babesia ovis, B. motasi, B. crassa [comprising strains B. crassa (Iran) and B. crassa (Turkey)] and several novel species: Theileria sp. 1 (China), Theileria sp. 2 (China) and Babesia sp. (China), [comprising strain Babesia sp. (Lintan), and Babesia sp. (Ningxian)] as defined previously. Based on the ascertained gene variations a reverse line blotting (RLB) assay was developed enabling direct, concurrent, highly specific and sensitive identification of virtually all presently known ovine/caprine piroplasm species. All probes bound to their respective target sequence only, therefore, no cross-reaction was observed resulting in clear recognition of either individual strains, species or groups. No signal was observed when ovine and caprine genomic DNA was used as the control, demonstrating that the signals are due to the presence of parasite DNA in investigated samples. Furthermore, the sensitivity of RLB could be considerably enhanced to detect a parasitemia level of at least 10(-12)% by reamplification of PCR products (nested PCR) thereby substantially increasing the possibility of identifying carrier animals.

摘要

在绵羊/山羊梨形虫物种的小核糖体RNA基因的高变区4(V4区)内鉴定出特征性序列特征,这些物种包括莱氏泰勒虫、绵羊泰勒虫、分离泰勒虫、绵羊巴贝斯虫、莫氏巴贝斯虫、粗巴贝斯虫[包括粗巴贝斯虫(伊朗)和粗巴贝斯虫(土耳其)菌株]以及几个新物种:泰勒虫1号种(中国)、泰勒虫2号种(中国)和巴贝斯虫种(中国)[包括巴贝斯虫种(临潭)和巴贝斯虫种(宁县)菌株],如先前所定义。基于确定的基因变异,开发了一种反向线杂交(RLB)检测方法,可直接、同时、高度特异性且灵敏地鉴定几乎所有目前已知的绵羊/山羊梨形虫物种。所有探针仅与各自的靶序列结合,因此,未观察到交叉反应,从而能够清晰识别单个菌株、物种或类群。以绵羊和山羊基因组DNA作为对照时未观察到信号,这表明信号是由于被调查样本中存在寄生虫DNA所致。此外,通过对PCR产物进行再扩增(巢式PCR),RLB的灵敏度可显著提高,以检测至少10(-12)%的寄生虫血症水平,从而大大增加识别携带动物的可能性。

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