贝类派琴虫原位杂交检测方法的建立与应用

Development and Application of an In-situ Hybridization Assay for Detection of Perkinsus spp. in Clams

下载PDF

导出

摘要本研究选择派琴虫特异性引物PerkITS85和PerkITS750的PCR扩增产物进行地高辛标记制备探针,探索建立了派琴虫的组织切片原位杂交检测方法,并应用该方法检测我国黄海海域采集的贝类样品。研究结果表明,PerkITS85和PerkITS750的PCR扩增产物大小为673bp,利用随机引物扩增法制备的派琴虫地高辛标记探针特异性好,与包纳米虫和尼氏单孢子虫均无交叉反应。以世界动物卫生组织(OIE)推荐的瑞氏液体羟基乙酸盐(RFTM)培养法为金标准对本研究建立的原位杂交检测方法进行评价,其诊断敏感性(Dse)为90.9%,诊断特异性(Dsp)为100%。实际检测应用表明本研究所建立的派琴虫原位杂交检测方法是一种有效的派琴虫检测方法,可以应用于派琴虫病的检测。 In this study,the conserved ITS fragment of Perkinsus was amplified by PCR using the genus-specific PerkITS85 and PerkITS750 as primers. The purified amplicons were digoxigenin-labeled and used as probes in the in-situ hybridizatio（SH）assay. Clam samples from the Yellow Sea were collected and screened by the developed ISH assay to confirm the perkinsus infection status. Results showed that a 673 bp fragment of perkinsus ITS gene was successfully amplified by PCR. The digoxigenin-labeled probe showed high specificity, without cross-reaction with Bonamia ostreae and Haplosporidium nelsoni and other aquatic parasites. The OIE recommended Ray＇s fluid thioglycollate medium（RFTM）culture assay was used as gold standard to evaluate the developed ISH assay,and it was found that the DSe of the ISH assay was 90.9%,and the DSp was 100%. Field application indicated that the developed ISH assay was an effective detection method for perkinsus and could be applied to perkinsus detection.

作者王彩霞冯春燕袁向芬邓俊花王宗祥吴绍强

机构地区中国检验检疫科学研究院动物检疫研究所内蒙古农业大学

出处《中国动物检疫》 CAS 2014年第6期79-83,共5页 China Animal Health Inspection

关键词贝类派琴虫原位杂交 RFTM 检测 clam Perkinsus in-situ hybridization Ray＇s fluid thioglycollate medium（RFTM） culture assay detection

分类号 S944.344 [农业科学—水产养殖]

引文网络
相关文献

参考文献17

1Bower S M, Mcgladdery S E, Price I M. Synopsis of infections diseases and parasites of commercially exploited shellfish [J]. Annu Rev Fish Dis, 1994, 4: 1-199.
2Wu S Q, Wang C X, Lin X M, et al. Infection prevalence and phylogenetic analysis of Perkinsus olseni in Ruditapes philippinarum from East China[J]. Dis Aquat Org, 2011, 96 ( 1 ): 55-60.
3Dungan C F, Roberson B S. Binding specificities ofmono- and polyclonal antibodies to the protozoan oyster pathogen Perkinsus marinus[J]. Dis Aquat Org, 1993, 15( 1 ): 9-22.
4Bushek D, Dungan C F, Lewitus A J. Serological affinities of the oyster pathogen Perkinsus marinus (Apicomplexa) with some dinoflagellates (Dinophyceae)[J]. J Eukaryot Microbiol, 2002, 49( 1 ): 11-16.
5Robledo J A F, Gauthier J D, Coss C A, et al. Species- specificity and sensitivity of a PCR-based assay for Perkinsus marinus in the eastern oyster, Crassostrea virginica: a comparison with the fluid thioglycollate assay[J]. J Parasitol, 1998, 84(6): 1237-1244.
6Gall J G, Pardue M L. Formation and detection of RNA-DNA hybrid molecules in cytological preparations[J]. Proc Natl Acad Sci U S A, 1969, 63(2): 378-383.
7Carnegie R, Barber B J, Culloty S C, et al. Development of a PCR assay for detection of the oyster pathogen Bonamia ostreae and support for its inclusion in the Haplosporidia[J]. Dis Aquat Org, 2000, 42(3), 199-206.
8Stokes N A, Siddall M E, Burreson E M. Detection of Haplosporidium nelsoni (Haplosporidia, Haplosporidiidae) in oysters by PCR amplification[J]. Dis Aquat Org, 1995, 23( 1 ): 145-152.
9Moss JA, Burreson E M, Reece K S. Advanced Perkinsus marinus infections in Crassostrea ariakensis maintained under laboratory conditions[J]. J Shellfish Res, 2006, 25( 1 ): 65-72.
10Audemard C, Reece K S, Burreson E M. Real-time PCR for the detection and quantification of the protistan parasite Perkinsus marinus in environmental waters[J]. Appl Envrion Microbiol, 2004, 70( 11 ).. 6611-6618.

二级参考文献28

1姚鑫,杨汉春,郭鑫,陈艳红,查振林.猪圆环病毒2型原位杂交检测技术的建立与应用[J].畜牧兽医学报,2007,38(2):169-174. 被引量：14
2WOOD J L, ANDREWS J D. Haplosporidium costale (Sporozoa) associated with a disease of Virginia oysters [ J ]. Science, 1962 (136) :710-711.
3ANDREWS J D. Epizootiology of diseases of oysters ( Crassostrea virginica), and parasites of associated organisms in eastern North America [ J ]. Helgol nder Meeresuntersuchungen, 1984 ( 27 ) : 149-166.
4ANDREWS J D. Haplosporidium costale disease of oysters [ A ]. Disease Diagnosis and Control in North American Marine Aquaculture [ C ]. Elsevier, Amsterdam, 1988:296-299.
5SUNILA I, STOKES N A, SMOLOWITZ R, et al. Haplosporidium costale (seaside organism), a parasite of the eastern oyster, is present in Long Island Sound [ J]. Journal of Shellfish Research, 2002(21 ) :113-118.
6ANDREWS J D,WOOD J L, HOESE H D. Oyster mortality studies in Virginia :III. Epizootiology of a disease caused by Haplosporidium costale [ J ]. Journal of Insect Pathology, 1962,4 ( 3 ) : 327- 343.
7BURRESON E M, FORD S E. A review of recent information on the Haplosporidia, with special reference to Haplosporidium nelsoni ( MSX disease) [ J]. Aquatic Living Resource, 2004 ( 17 ) : 499 -517.
8CHU F L,BURRESON E M,ZHANG F S,et al. An unidentified haplosporidian parasite of bay scallop Argopecten irradians cultured in the Shandong and Liaoning provinces of China[ J]. Disease of Aquatic Organisms, 1996 ( 25 ) : 155-158.
9FORD S E. Effect of repeated hemolymph sampling on growth, mortality, hemolymph protein and parasitism of oysters, Crassostrea virginica [ J]. Physiology, 1986,85A :465-470.
10STOKES N A, BURRESON E M. Differential diagnosis of mixed Haplosporidium costale and Haplosporidium nelsoni infections in the eastern oyster, Crassostrea virginica, using DNA probes [ J ]. Shellfish Research ,2001 ( 20 ) :207-213.

共引文献16

1李雪梅,程安春,汪铭书,刘伍梅,张平英,豆文波,陈希文.寡核苷酸探针原位检测石蜡切片中PRRSV核酸[J].中国兽医学报,2006,26(4):350-353. 被引量：6
2卢慎.应用间接原位PCR诊断弓形虫淋巴结炎[J].江苏大学学报（医学版）,2008,18(1):70-72. 被引量：7
3李雪梅,程安春,汪铭书.人工感染仔猪猪生殖与呼吸综合征病毒的核酸分布规律[J].中国兽医科学,2008,38(4):278-282. 被引量：4
4马晓明,孟晓丽,殷国荣,刘红丽,申金雁.RNA原位杂交法动态观察弓形虫速殖子对BALB/c小鼠小肠黏膜的黏附及侵入[J].中国寄生虫学与寄生虫病杂志,2008,26(4):272-276. 被引量：3
5卢慎.应用免疫组化、原位杂交及间接原位PCR诊断弓形虫淋巴结炎[J].中国实验诊断学,2008,12(10):1305-1307. 被引量：1
6卢慎.应用3种方法诊断弓形虫淋巴结炎[J].世界感染杂志,2008,8(5):375-378. 被引量：3
7孟晓丽,马晓明,殷国荣,刘红丽,殷丽天,申金雁,王海龙.RNA原位杂交法检测灌胃接种弓形虫速殖子小鼠体内虫体的早期动态分布[J].中国寄生虫学与寄生虫病杂志,2010,28(2):139-142. 被引量：1
8赵晋英,黄泽智,李艳伟,侯玉英,王秀虎,何跃华,孙友平.孕期弓形虫感染对胎盘的入侵和病理损害的研究[J].热带医学杂志,2010,10(12):1384-1386. 被引量：1
9刘斌,李海龙,韩英.原位杂交技术在水产动物育种与疾病诊断中的应用[J].水产学杂志,2011,24(2):53-56. 被引量：2
10常志尚,张忠广,宫玉香.寡核苷酸探针RNA原位杂交法检测肺孢子虫的研究[J].热带医学杂志,2011,11(10):1115-1117. 被引量：1

1李永才,张宝才,刘再胜,王芳.二羟基乙酸盐比色法测定饲料中色氨酸的含量[J].饲料工业,1996,17(12):34-35.
2谢丽基,谢芝勋,庞耀珊,刘加波,邓显文,谢志勤,范晴,罗思思.中国沿海主要养殖贝类四种原虫病流行病学的调查研究[J].基因组学与应用生物学,2012,31(6):559-566. 被引量：3
3张万坡,程国富,谷长勤,李德学,宋念华,毕丁仁,胡薛英,胡思顺,胡智斌.H9N2亚型禽流感病毒原位杂交检测方法的建立[J].中国兽医学报,2005,25(4):371-373. 被引量：7
4苏威.大米生虫后怎么办[J].新农村,2003(11):22-22.
5王勤,刘晓飞,冯春燕,翟新验,周智,吴绍强,李晓琳,仇松寅,刘丹丹,林祥梅.蓝耳病病毒抗体ELISA检测试剂盒的“两步法”评价[J].中国动物检疫,2016,33(1):71-75. 被引量：1
6杨化林,李靖.乳山市渔业部门放生罕见鲈鳗[J].河北渔业,2012(6):69-69.
7王勤,刘晓飞,江育林,母连志,丁壮,林祥梅.传染病诊断方法的验证[J].中国动物检疫,2015,32(8):53-55.
8唐勇,陈焕春,覃雅丽,何启盖,金梅林,吴斌,刘正飞.猪伪狂犬病gE-ELISA鉴别诊断方法的建立及初步应用[J].农业生物技术学报,2004,12(6):635-638. 被引量：6
9吕玲,何建国,邓敏,翁少萍,左涛.核酸探针原位杂交检测白斑综合症病毒的组织特异性[J].热带海洋,2000,19(4):86-91. 被引量：12
10赵玉龙,焦玉兰,郁宏伟,李莹洁,杨保收.一种猪圆环病毒Ⅱ型ELISA抗体检测试剂盒的临床应用[J].中国兽药杂志,2011,45(3):31-34. 被引量：3

中国动物检疫

2014年第6期

浏览历史

内容加载中请稍等...

贝类派琴虫原位杂交检测方法的建立与应用

参考文献17

二级参考文献28

共引文献16

相关作者

相关机构

相关主题

浏览历史