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在亚马逊东部河口地区养殖的牡蛎中检测刚地弓形虫。

Detection of Toxoplasma gondii in Crassostrea spp. oysters cultured in an estuarine region in eastern Amazon.

作者信息

Monteiro Thamillys R M, Rocha Katarine S, Silva Jacqueline, Mesquita Gleiciane S S, Rosário Marcely K S, Ferreira Maeli F S, Honorio Betsy E T, Melo Hugo F R, Barros Flávia N L, Scofield Alessandra, Abel Isis, Moraes Carla C G

机构信息

Laboratory of Zoonoses and Public Health (LZSP), Graduate Program in Animal Health in the Amazon, Institute of Veterinary Medicine, Federal University of Pará (UFPA), Castanhal, Pará, Brazil.

Faculty of Veterinary Medicine, Institute of Veterinary Medicine, Federal University of Pará (UFPA), Castanhal, Pará, Brazil.

出版信息

Zoonoses Public Health. 2019 May;66(3):296-300. doi: 10.1111/zph.12564. Epub 2019 Jan 27.

Abstract

The aim of the present study was to detect DNA of Toxoplasma gondii in Crassostrea spp. oysters cultured in the state of Pará, Brazil. A total of 400 oysters were directly collected from a fixed rack system. Gills, gastrointestinal tract (GIT) and intervalvular liquid were separated and grouped into pool samples of 10 animals, resulting in 40 samples each of gills, GIT and intervalvular liquid. DNA extraction was performed using a commercial kit, and T. gondii DNA was detected by nested PCR using the primers Toxo3 and Toxo4, which produced an amplification product of 155 bp of the T. gondii gene B1. Nucleotide sequencing was performed for positive samples, and the obtained sequences were identified by comparison with sequences in GenBank. The DNA of T. gondii was detected in 5.8% (7/120) of the pool samples, of which 7.5% (3/40) was in the GIT, 5% (2/40) in the gills, and 5% (2/40) was in the intervalvular liquid. The obtained sequences presented 100% identity and overlap with T. gondii DNA sequences. This is the report of detection of T. gondii DNA in oysters from genus Crassostrea spp. originating from the state of Pará, eastern Amazon.

摘要

本研究的目的是检测巴西帕拉州养殖的牡蛎属牡蛎中刚地弓形虫的DNA。总共从一个固定架系统中直接采集了400只牡蛎。将鳃、胃肠道(GIT)和瓣间液分离,并将其分成每组10只动物的混合样本,从而得到40个鳃、GIT和瓣间液样本。使用商业试剂盒进行DNA提取,并使用引物Toxo3和Toxo4通过巢式PCR检测刚地弓形虫DNA,该引物产生了刚地弓形虫基因B1的155 bp扩增产物。对阳性样本进行核苷酸测序,并通过与GenBank中的序列进行比较来鉴定获得的序列。在5.8%(7/120)的混合样本中检测到了刚地弓形虫DNA,其中7.5%(3/40)在GIT中,5%(2/40)在鳃中,5%(2/40)在瓣间液中。获得的序列与刚地弓形虫DNA序列具有100%的同一性和重叠。这是关于来自亚马逊东部帕拉州的牡蛎属牡蛎中检测到刚地弓形虫DNA的报告。

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