基于novel-miR1检测家兔豆状囊尾蚴感染的滚环扩增方法的建立和应用

doi:10.12140/j.issn.1000-7423.2023.03.005

中国寄生虫学与寄生虫病杂志 ›› 2023, Vol. 41 ›› Issue (3): 294-299.doi: 10.12140/j.issn.1000-7423.2023.03.005

基于novel-miR1检测家兔豆状囊尾蚴感染的滚环扩增方法的建立和应用

陈国梁¹(), 王立群¹, 李艳萍¹, 刘婷丽¹, 李红¹, 张少华¹, 骆学农¹, 强文军²^,^*()

1 中国农业科学院兰州兽医研究所，家畜疫病病原生物学国家重点实验室，兰州 730046
2 甘肃省武威市凉州区畜牧兽医技术推广中心，武威 733000

收稿日期:2022-08-31 修回日期:2022-11-04 出版日期:2023-06-30 发布日期:2023-06-21
通讯作者: *强文军（1971-）男，高级兽医师，从事动物疫病防控研究。E-mail：1145303446@qq.com
作者简介:陈国梁（1995-），男，硕士研究生，从事人兽共患病与兽医公共卫生研究。E-mail：glchen2019@163.com
基金资助:
国家自然科学基金(32072889)

Establishment and application of a rolling circle amplification method based on novel-miR1 for detection of Cysticercus pisiformis infection in rabbit

CHEN Guoliang¹(), WANG Liqun¹, LI Yanping¹, LIU Tingli¹, LI Hong¹, ZHANG Shaohua¹, LUO Xuenong¹, QIANG Wenjun²^,^*()

1 State Key Laboratory of Veterinary Etiological Biology/Lanzhou Veterinary Research Institute, Chinese Academy of Agricultural Sciences, Lanzhou 730046, Gansu, China
2 Animal Husbandry and Veterinary Technology Extension Center, Liangzhou District, Wuwei 733000, Gansu, China

Received:2022-08-31 Revised:2022-11-04 Online:2023-06-30 Published:2023-06-21
Contact: *E-mail: 1145303446@qq.com
Supported by:
National Natural Science Foundation(32072889)

摘要/Abstract

摘要：

目的建立检测家兔豆状囊尾蚴感染的滚环扩增（RCA）方法。方法以家兔血清中豆状囊尾蚴来源的novel-miR1为诊断靶标，设计连接序列和锁式探针，并对连接序列和锁式探针的比例、反应时间、酶用量、dNTP用量以及扩增反应时间等5个重要条件进行优化，建立检测豆状囊尾蚴感染的RCA方法。将novel-miR1标准品倍比稀释为1 fmol/L至100 nmol/L的9个不同浓度的样品，评价RCA方法的灵敏度。用优化后的RCA方法分别检测健康家兔和豆状囊尾蚴感染家兔血清miRNA各20份（实验室保存样品），并通过受试者工作特征（ROC）曲线分析其敏感性和特异性。20只雌性家兔每只经口感染1 000个豆状带绦虫虫卵，采集感染前和感染后每个月的家兔血样制备血清miRNA，用优化后的RCA方法进行检测，评价其应用效果。结果电泳结果显示，RCA扩增产物的DNA停留在加样孔中，形成一条明亮条带。反应条件优化试验结果显示，连接序列浓度为2 μmol/L、锁式探针浓度为1 μmol/L（连接序列和锁式探针的比为2∶1）、T4 DNA连接酶为350 U、连接180 min时连接效率最高。在100 μl的扩增体系中，dNTP浓度为0.5 μmol/L，扩增240 min时，RCA扩增效果最佳。优化后RCA的最低检测浓度为10 pmol/L。RCA检测健康家兔和豆状囊尾蚴感染家兔血清miRNA样品的平均荧光值分别为53.298 ± 1.707和97.498 ± 5.892，差异有统计学意义（t = 7.206，P < 0.01）。ROC分析结果显示，当阳性临界值为61.69时，RCA方法的敏感性和特异性均为95%，AUC为0.955 0，似然比为19.00。RCA检测豆状囊尾蚴感染后不同时间的家兔血清miRNA结果显示，20份感染前的血清中19份检测结果为阴性，1份为阳性；感染后1个月的血清中，17份为阳性，2份为疑似，1份为阴性；感染后2个月的血清，1份为阴性，其余为阳性；感染后3个月的血清，3份为阴性，其余为阳性。结论建立了检测家兔豆状囊尾蚴感染的RCA方法，该方法在豆状囊尾蚴感染后3个月内的家兔血清中检出novel-miR1，具有良好的应用潜力。

关键词: 豆状囊尾蚴病, novel-miR1, 滚环扩增

Abstract:

Objective To establish a rolling circle amplification (RCA) method for detection of Cysticercus pisiformis infection in rabbits. Methods The novel-miR1 derived from C. pisiformis in rabbit serum served as the diagnostic target to establish an RCA diagnostic method for cysticercosis pisiformis fection in rabbit. To establish the RCA method, ligation sequence and the locking probe sequence were designed, and five important reaction conditions were optimized, including the ratio of ligation sequence and padlock probe, ligation reaction time, ligase dosage, amplification reaction time, and dNTP dosage. The sensitivity of the RCA method was assessed, the novel-miR1 standard was serially diluted into 9 samples of different concentrations ranging from 1 fmol/L to 100 nmol/L. The sensitivity and specificity of the optimized RCA methods were assayed using the serum miRNA from 20 healthy rabbits and 20 C. pisiformis infected rabbits (Laboratory preserved samples), and analyzed by the receiver operating characteristic curve (ROC curve) method. To evaluate the application effectiveness of the RCA, 20 female rabbits were infected by gavage with 1 000 eggs of T. pisiformis for collection of serum every month post-infection, which were used to prepare miRNA for application in RCA method under optimized condition. Results The agarose gel electrophoresis results showed that the RCA amplification products remained in the sampling wells of agarose gel, forming a bright band. The tests to optimize RCA condition indicated that the concentration of ligation sequence was 2 μmol/L, padlock probe was 1 μmol/L (ratio of ligation sequence and padlock probe was 2∶1), T4 DNA ligase was 350 U, and the efficacy of ligation reaction was found the highest when ligating for 180 min. The optimal amplification reaction system was 0.5 μmol/L dNTP and amplification reacted 240 min in 100 μl amplification reaction system. Lastly, the RCA method limit of detection was proved to be 10 pmol/L. The RCA method detected showed that the average serum miRNA fluorescence intensity of the samples from healthy rabbits and C. pisiformis infected rabbits were 53.298 ± 1.707 and 97.498 ± 5.892, respectively, which was statistically significant (t = 7.206, P < 0.01). ROC curve showed that the RCA method cut-off value was 61.69 and both sensitivity and specificity were 95%, the area under the curve (AUC) is 0.955 0, likelihood ratio was 19.00. Using the RCA method to detect 20 healthy rabbits’ serum miRNA found 19 samples were negative and 1 positive. The results of RCA detection of the C. pisiformis infected rabbits serum miRNA at different times found that 17 were positive, 2 were suspected, 1 were negative 1 month post-infection. One was negative, and 19 were positive 2 mouths post-infection. Three were negative, and 17 were positive 3 months post-infection. Conclusion An RCA method was established for detecting C. pisiformis infection in rabbits. It was demonstrated that novel-miR1 could be detected by RCA in the serum of rabbits within 3 months post-infection of C. pisiformis, showing good application potential.

Key words: Cysticercosis pisiformis, Novel-miR1, Rolling circle amplification

中图分类号:

R532.39

陈国梁, 王立群, 李艳萍, 刘婷丽, 李红, 张少华, 骆学农, 强文军. 基于novel-miR1检测家兔豆状囊尾蚴感染的滚环扩增方法的建立和应用[J]. 中国寄生虫学与寄生虫病杂志, 2023, 41(3): 294-299.

CHEN Guoliang, WANG Liqun, LI Yanping, LIU Tingli, LI Hong, ZHANG Shaohua, LUO Xuenong, QIANG Wenjun. Establishment and application of a rolling circle amplification method based on novel-miR1 for detection of Cysticercus pisiformis infection in rabbit[J]. Chinese Journal of Parasitology and Parasitic Diseases, 2023, 41(3): 294-299.

图/表 3

参考文献 30

[1]	Yang DY, Yang GY. Research progress on rabbit cysticercosis[J]. China Animal Husb ＆ Vet Med, 2015, 42(4): 1015-1020. (in Chinese)
	(杨德英, 杨光友. 兔豆状囊尾蚴病研究进展[J]. 中国畜牧兽医, 2015, 42(4): 1015-1020.)
[2]	Wang LJ, Wang LQ, Liu TL, et al. Polyclonal antibody preparation, tissue localization and activity of serine protease inhibitor serpin of Cysticercus pisiformis[J]. Chin J Parasitol Parasit Dis, 2020, 38(5): 595-601. (in Chinese)
	(王莉杰, 王立群, 刘婷丽, 等. 豆状囊尾蚴丝氨酸蛋白酶抑制剂(serpin)的多抗制备、组织分布及活性研究[J]. 中国寄生虫学与寄生虫病杂志, 2020, 38(5): 595-601.)
[3]	Pan YQ, Kong LY, Li P, et al. Identification and 18S DNA sequence analysis of a new type no-hook Cysticercus pisiformis[J]. Chin J Animal Vet Sci, 2019, 50(11): 2283-2289. (in Chinese)
	(潘耀谦, 孔令芸, 李鹏, 等. 一种新型无钩豆状囊尾蚴的鉴定和18S DNA序列分析[J]. 畜牧兽医学报, 2019, 50(11): 2283-2289.)
[4]	Stancampiano L, Ravagnan S, Capelli G, et al. Cysticercosis by Taenia pisiformis in brown hare (Lepus europaeus) in northern Italy: epidemiologic and pathologic features[J]. Int J Parasitol Parasites Wildl, 2019, 9: 139-143. doi: 10.1016/j.ijppaw.2019.04.004
[5]	Remesar S, Castro-Scholten S, Jiménez-Martín D, et al. Spatiotemporal monitoring of Cysticercus pisiformis in European wild rabbit (Oryctolagus cuniculus) in Mediterranean ecosystems in southern Spain[J]. Prev Vet Med, 2021, 197: 105508. doi: 10.1016/j.prevetmed.2021.105508
[6]	Hajipour N, Zavarshani M. Ectoparasites and endoparasites of New Zealand white rabbits from north west of Iran[J]. Iran J Parasitol, 2020, 15(2): 266-271. pmid: 32595718
[7]	Wang LQ. Characteristics of exosomes from Cysticercus pisiformis and their mechanism on regulating macrophage polarization[D]. Beijing: Chinese Academy of Agricultural Sciences, 2020: 2. (in Chinese)
	(王立群. 豆状囊尾蚴外泌体的特征及其对巨噬细胞极化的调节机制[D]. 北京: 中国农业科学院, 2020: 2.)
[8]	Tian QH. The changes of antibodies in rabbits infected with Cysticercus pisiformis[J]. Chin J Rabbit Farming, 2021(1): 12-15. (in Chinese)
	(田启会. 家兔感染豆状囊尾蚴后抗体的消长[J]. 中国养兔杂志, 2021(1): 12-15.)
[9]	Liu CL, Yang HR, Shi WY, et al. microRNA-mediated regulation of T helper type 17/regulatory T-cell balance in autoimmune disease[J]. Immunology, 2018, 155(4): 427-434. doi: 10.1111/imm.12994 pmid: 30133700
[10]	Yadav SK, Pandey A, Sarkar S, et al. Identification of altered blood microRNAs and plasma proteins in a rat model of Parkinson’s disease[J]. Mol Neurobiol, 2022, 59(3): 1781-1798. doi: 10.1007/s12035-021-02636-y
[11]	Zhao ZT, Zhu AN, Bhardwaj M, et al. Fecal microRNAs, fecal microRNA panels, or combinations of fecal microRNAs with fecal hemoglobin for early detection of colorectal cancer and its precursors: a systematic review[J]. Cancers, 2021, 14(1): 65. doi: 10.3390/cancers14010065
[12]	Chen QL, Zhang JQ, Zheng T, et al. The role of microRNAs in the pathogenesis, grading and treatment of hepatic fibrosis in schistosomiasis[J]. Parasit Vectors, 2019, 12(1): 611. doi: 10.1186/s13071-019-3866-0 pmid: 31888743
[13]	Rouas R, Merimi M, Najar M, et al. Human CD8⁺ CD25⁺ CD127 low regulatory T cells: microRNA signature and impact on TGF-β and IL-10 expression[J]. J Cell Physiol, 2019, 234(10): 17459-17472. doi: 10.1002/jcp.v234.10
[14]	Cheong JK, Tang YC, Zhou LH, et al. Advances in quantifying circulatory microRNA for early disease detection[J]. Curr Opin Biotechnol, 2022, 74: 256-262. doi: 10.1016/j.copbio.2021.12.007
[15]	Tian B, Qiu Z, Ma J, et al. On-particle rolling circle amplification-based core-satellite magnetic superstructures for microRNA detection[J]. ACS Appl Mater Interfaces, 2018, 10(3): 2957-2964. doi: 10.1021/acsami.7b16293
[16]	Deng XJ, Qin SS, Chen YQ, et al. B-RCA revealed circulating miR-33a/b associates with serum cholesterol in type 2 diabetes patients at high risk of ASCVD[J]. Diabetes Res Clin Pract, 2018, 140: 191-199. doi: 10.1016/j.diabres.2018.03.024
[17]	Yao MD, Lv XF, Deng YL, et al. Specific and simultaneous detection of micro RNA 21 and let-7a by rolling circle amplification combined with lateral flow strip[J]. Anal Chim Acta, 2019, 1055: 115-125. doi: S0003-2670(18)31489-2 pmid: 30782362
[18]	Treerattrakoon K, Jiemsakul T, Tansarawiput C, et al. Rolling circle amplification and graphene-based sensor-on-a-chip for sensitive detection of serum circulating miRNAs[J]. Anal Biochem, 2019, 577: 89-97. doi: S0003-2697(18)30941-2 pmid: 31029676
[19]	Chen GL, Wang LQ, Liu TL, et al. Identification and expression profiling of circulating microRNAs in serum of Cysticercus pisiformis-infected rabbits[J]. Genes, 2021, 12(10): 1591. doi: 10.3390/genes12101591
[20]	Zhang JJ. Methodological study on rolling circle amplification detection of miR-93-5p[D]. Shenyang: China Medical University, 2019: 8-10. (in Chinese)
	(张佳佳. 滚环扩增检测miR-93-5p的方法学研究[D]. 沈阳: 中国医科大学, 2019: 8-10.)
[21]	Mu Y, McManus DP, Gordon CA, et al. Parasitic helminth-derived microRNAs and extracellular vesicle cargos as biomarkers for helminthic infections[J]. Front Cell Infect Microbiol, 2021, 11: 708952. doi: 10.3389/fcimb.2021.708952
[22]	Hoy AM, Lundie RJ, Ivens A, et al. Parasite-derived microRNAs in host serum as novel biomarkers of helminth infection[J]. PLoS Negl Trop Dis, 2014, 8(2): e2701. doi: 10.1371/journal.pntd.0002701
[23]	Cai PF, Gobert GN, You H, et al. Circulating miRNAs: potential novel biomarkers for hepatopathology progression and diagnosis of schistosomiasis japonica in two murine models[J]. PLoS Negl Trop Dis, 2015, 9(7): e0003965. doi: 10.1371/journal.pntd.0003965
[24]	Mu Y, Cai PF, Olveda RM, et al. Parasite-derived circulating microRNAs as biomarkers for the detection of human Schistosoma japonicum infection[J]. Parasitology, 2020, 147(8): 889-896. doi: 10.1017/S0031182019001690
[25]	Cao DP, Jiang BF, Zhang YG, et al. microRNA-125b-5p is a promising novel plasma biomarker for alveolar echinococcosis in patients from the southern Province of Qinghai[J]. BMC Infect Dis, 2021, 21(1): 246. doi: 10.1186/s12879-021-05940-z pmid: 33678159
[26]	Chen XG, Li ZY, Maleewong W, et al. Serum aca-mir-146a is a potential biomarker for early diagnosis of Angiostrongylus cantonensis infection[J]. Parasitol Res, 2014, 113(9): 3221-3227. doi: 10.1007/s00436-014-3984-8
[27]	Yang DY, Chen L, Xie Y, et al. Expression and immunolocalisation of TpFABP as a candidate antigen for the serodiagnosis of rabbit Taenia pisiformis cysticercosis[J]. Parasite, 2013, 20: 53. doi: 10.1051/parasite/2013053
[28]	Yang DY, Chen L, Wu XH, et al. Expression of the Tpanxb1 gene from Taenia pisiformis and its potential diagnostic value by dot-ELISA[J]. J Parasitol, 2014, 100(2): 246-250. doi: 10.1645/13-304.1
[29]	Chen L, Yang DY, Gu XB, et al. Evaluation of a novel dot-ELISA assay utilizing a recombinant protein for the effective diagnosis of Taenia pisiformis larval infections[J]. Vet Parasitol, 2014, 204(3/4): 214-220. doi: 10.1016/j.vetpar.2014.05.021
[30]	Wang LJ, Zhang SH, Mao L, et al. Development of indirect ELISA for the diagnosis of Cysticercus pisiformis infection based on recombinant serpin[J]. Chin Vet Sci, 2018, 48(4): 443-449. (in Chinese)
	(王莉杰, 张少华, 毛立, 等. 基于serpin重组蛋白的豆状囊尾蚴病间接ELISA诊断方法的初步建立[J]. 中国兽医科学, 2018, 48(4): 443-449.)

基于novel-miR1检测家兔豆状囊尾蚴感染的滚环扩增方法的建立和应用

Establishment and application of a rolling circle amplification method based on novel-miR1 for detection of Cysticercus pisiformis infection in rabbit

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