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鹅胚适应型番鸭细小病毒疫苗株FZ91 - 30感染性克隆的构建与测序

Construction and sequencing of an infectious clone of the goose embryo-adapted Muscovy duck parvovirus vaccine strain FZ91-30.

作者信息

Wang Jianye, Huang Yu, Zhou Mingxu, Hardwidge Philip R, Zhu Guoqiang

机构信息

College of Veterinary Medicine, Yangzhou University, 48 Wenhui East Road, 225009, Yangzhou, Peoples' Republic of China.

College of Veterinary Medicine, Kansas State University, Manhattan, KS, USA.

出版信息

Virol J. 2016 Jun 21;13:104. doi: 10.1186/s12985-016-0564-9.

Abstract

BACKGROUND

Muscovy duck parvovirus (MDPV) is the etiological agent of Muscovy duckling parvoviral disease, which is characterized by diarrhea, locomotive dysfunction, stunting, and death in young ducklings, and causes substantial economic losses in the Muscovy duck industry worldwide. FZ91-30 is an attenuated vaccine strain that is safe and immunogenic to ducklings, but the genomic information and molecular mechanism underlining the attenuation are not understood.

METHODS

The FZ91-30 strain was propagated in 11-day-old embryonated goose eggs, and viral particles were purified from the pooled allantoic fluid by differential centrifugation and ultracentrifugation. Single-stranded genomic DNA was extracted and annealed to form double-stranded DNA. The dsDNA digested with NcoI resulted two sub-genomic fragments, which were then cloned into the modified plasmid pBluescript II SK, respectively, generating plasmid pBSKNL and pBSKNR. The sub-genomic plasmid clones were sequenced and further combined to construct the plasmid pFZ that contained the entire genome of strain FZ91-30. The complete genome sequences of strain FM and YY and partial genome sequences of other strains were retrieved from GenBank for sequence comparison. The plasmid pFZ containing the entire genome of FZ91-30 was transfected in 11-day-old embryonated goose eggs via the chorioallantoic membranes route to rescue infectious virus. A genetic marker was introduced into the rescued virus to discriminate from its parental virus.

RESULTS

The genome of FZ91-30 consists of 5,131 nucleotides and has 98.9 % similarity to the FM strain. The inverted terminal repeats (ITR) are 456 nucleotides in length, 14 nucleotides longer than that of Goose parvovirus (GPV). The exterior 415 nucleotides of the ITR form a hairpin structure, and the interior 41 nucleotides constitute the D sequence, a reverse complement of the D' sequence at the 3' ITR. Amino acid sequence alignment of the VP1 proteins between FZ91-30 and five pathogenic MDPV strains revealed that FZ91-30 had five mutations; two in the unique region of the VP1 protein (VP1u) and three in VP3. Sequence alignment of the Rep1 proteins revealed two amino acid alterations for FZ91-30, both of which were conserved for two pathogenic strains YY and P. Transfection of the plasmid pFZ in 11-day-old embryonated goose eggs resulted in generation of infectious virus with similar biological properties as compared with the parental strain.

CONCLUSIONS

The amino acid mutations identified in the VP1 and Rep1 protein may contribute to the attenuation of FZ91-30 in Muscovy ducklings. Plasmid transfection in embryonated goose eggs was suitable for rescue of infectious MDPV.

摘要

背景

番鸭细小病毒(MDPV)是番鸭雏细小病毒病的病原体,其特征为雏鸭腹泻、运动功能障碍、发育迟缓及死亡,给全球番鸭养殖业造成重大经济损失。FZ91 - 30是一种减毒疫苗株,对雏鸭安全且具有免疫原性,但减毒的基因组信息和分子机制尚不清楚。

方法

FZ91 - 30株在11日龄鹅胚中增殖,通过差速离心和超速离心从合并的尿囊液中纯化病毒颗粒。提取单链基因组DNA并退火形成双链DNA。用NcoI消化双链DNA产生两个亚基因组片段,然后分别克隆到修饰的质粒pBluescript II SK中,构建质粒pBSKNL和pBSKNR。对亚基因组质粒克隆进行测序,并进一步组合构建包含FZ91 - 30株全基因组的质粒pFZ。从GenBank检索FM和YY株的全基因组序列及其他株的部分基因组序列进行序列比较。将包含FZ91 - 30全基因组的质粒pFZ通过绒毛尿囊膜途径转染到11日龄鹅胚中以拯救感染性病毒。在拯救的病毒中引入一个遗传标记以与亲代病毒区分。

结果

FZ91 - 30的基因组由5131个核苷酸组成,与FM株的相似性为98.9%。反向末端重复序列(ITR)长度为456个核苷酸,比鹅细小病毒(GPV)的长14个核苷酸。ITR外部的415个核苷酸形成发夹结构,内部的41个核苷酸构成D序列,是3' ITR处D'序列的反向互补序列。FZ91 - 30与5个致病性MDPV株的VP1蛋白氨基酸序列比对显示,FZ91 - 30有5个突变;2个位于VP1蛋白的独特区域(VP1u),3个位于VP3。Rep1蛋白的序列比对显示FZ91 - 30有2个氨基酸改变,这两个改变在两个致病性株YY和P中是保守的。将质粒pFZ转染到11日龄鹅胚中产生了与亲代株具有相似生物学特性的感染性病毒。

结论

在VP1和Rep1蛋白中鉴定出的氨基酸突变可能导致FZ91 - 30在番鸭雏中减毒。在鹅胚中进行质粒转染适合拯救感染性MDPV。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0cb6/4915054/0ffc518c2616/12985_2016_564_Fig1_HTML.jpg

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