A型流感病毒的反向遗传技术研究进展

A 型流感病毒基因组为单股负义RNA,分为8 个片段。反向遗传技术即从克隆的cDNA 产 生病毒的过程,是研究RNA 病毒、也是研究A 型流感病毒基因结构与功能的新技术。介绍了A 型流感病毒反向遗传技术的发展,完全以质粒为基础的新操作系统及其在研究病毒的生命周期、 致病性、产生基因修饰的疫苗候选株等方面的应用。     

合成病毒:对流感病毒研究的贡献

流感病毒是一种单股负链分节段RNA病毒。完全以质粒为基础的反向遗传学技术的建立和发展解决了利用cDNA克隆人工合成流感病毒的难题和技术障碍,并逐渐成为研究流感病毒及生产流感疫苗的重要基础和手段。重点综述了流感病毒反向遗传技术20多年来的发展过程,以及以质粒为基础的反向遗传操作系统在对流感病毒的生命周期、致病性的研究和生产疫苗等方面的巨大贡献。     

冠状病毒反向遗传技术的研究进展和应用

冠状病毒（Coronavirus,CoV）在分类上属于尼多病毒目、冠状病毒科、冠状病毒属,其基因组长度约为25 000 nt～30 000 nt。反向遗传技术可以针对RNA病毒的基因组进行突变,是研究病毒蛋白功能的有力工具,也是对毒力基因进行突变,构建减毒疫苗株的新型方法。冠状病毒反向遗传技术的建立和应用,推动了基因功能的研究和重组病毒疫苗的研发。本综述将介绍三种常见的冠状病毒反向遗传克隆技术,分别是基于痘病毒载体、基于细菌人工染色体（Bacterial artificial chromosome,BAC）载体和基于体外连接的反向遗传技术。传染性支气管炎病毒（Infectious bronchitis virus,IBV）是成功建立反向遗传系统的冠状病毒之一,本文对反向遗传技术在IBV中的研究和应用进行了介绍和讨论。     

弹状病毒基因组及功能基因研究进展

弹状病毒(rhabdovirus)是一类有包膜的负链RNA病毒,其宿主范围广泛,包括哺乳动物、鸟类、爬行动物、鱼类、昆虫以及植物等。大多数的弹状病毒是动植物重要病原,具有较强的致病性。解析病毒基因组及功能基因可为该病毒的致病机理、与宿主的互作机制以及疫苗研制等相关研究提供理论依据。本综述对弹状病毒的分类、基因组结构、结构蛋白及非结构蛋白功能等方面研究进行概述、归纳与简评,旨在为弹状病毒相关研究提供借鉴。     

RNA病毒的反向遗传学

反向遗传操作作为一种新兴技术在RNA病毒的研究中发挥着重要作用。本文介绍了RNA病毒反向遗传学的研究方法以及RNA病毒反向遗传技术的最新研究进展。     

反向遗传学技术及其在FMDV研究中的应用

反向遗传技术是一种新兴的分子生物学技术,已广泛应用于生命科学研究的各个领域。综述反向遗传技术研究进展,并讨论该技术在口蹄疫病毒研究中的应用。     

植物弹状病毒提纯技术的研究进展

弹状病毒(Rhabdoviruses)是一类由单分子负链单股RNA和蛋白质外壳组成的子弹形病毒,它包含一大批寄主范围不同的病毒成员,分类上属于弹状病毒科(Rhabdoviridae)。它们可分别侵染哺乳动物、鱼类、昆虫和植物。其中侵染植物的成员归为植物弹状病毒组,它们的颗粒呈棒状或子弹状,以棒状为主。到目前为止,对植物弹状病毒的研究与其他病毒相比是很不深入的,最主要的限制因素就是病毒本身的提纯。因此研究弹状病毒的提纯技术具有重要的意义。     

PB2 E627K对A/H6N1亚型禽流感病毒致病性的影响分析

目的利用A/H6N1亚型禽流感病毒的反向遗传平台,评估PB2 E627K对A/H6N1亚型禽流感病毒的致病性,探究A/H6N1流感病毒的致病性分子基础。方法通过A/H6N1亚型禽流感病毒A/Mallard/San-Jiang/275/2007株反向遗传操作系统和点突变技术拯救病毒rA/H6N1和PB2 E627K位点发生突变的rA/H6N1-627,两株拯救病毒分别以101EID50～106EID50的攻毒剂量人工感染BALB/c小鼠,通过体重变化、死亡率、病毒滴定等方面进行致病性分析。结果成功构建A/H6N1亚型禽流感病毒的反向遗传平台,rA/H6N1的8个基因片段完全源于A/H6N1的基因组,核苷酸序列及生物学特性与A/H6N1完全一致。rA/H6N1能够人工感染BALB/c小鼠,但不致死,对BALB/c小鼠呈现低致病性(MLD50>106.5EID50),病毒在小鼠体内的分布情况及各个脏器中的病毒滴度与A/H6N1保持一致;rA/H6N1-627能感染小鼠,引起小鼠体重下降,但不能引起所有106EID50组小鼠死亡,病毒能在小鼠的肺脏和脑部进行增殖。结论实验结果表明,在H5N1禽流感中发挥重要作用的PB2-E627K位点并非A/H6N1流感病毒的毒力决定因子。A/H6N1流感病毒致病性的分子基础还有待继续研究,该反向遗传操作系统和点突变技术的建立为研究该亚型流感病毒致病机制、传播机制及病毒基因功能奠定了基础,同时也为A/H6N1亚型禽流感病毒新型疫苗的研制开辟了新途径。     

内蒙古部分地区骆驼和羊寄生蜱虫病毒组学分析

为了解内蒙古地区蜱虫病毒组学的本底数据,采用病毒宏基因组学方法对在内蒙古阿拉善盟左旗、右旗和四子王旗地区3个采样点采集骆驼和羊体表寄生的1789只蜱虫样品进行病毒宏基因组学分析,并对特定病毒进行巢式PCR扩增和测序,通过Clustal W和MEGA7.0等生物信息学软件对获得的病毒基因序列进行遗传进化分析.数据显示,蜱虫样品携带包括植物、脊椎动物和非脊椎动物等来源的17个病毒科和一些未分类的病毒;其中,2株弹状病毒具有丰富的遗传多样性,与新疆地区和长江地区的弹状病毒的同源性达到98.5％和96.26％,提示蜱虫弹状病毒可能是通过羊和骆驼等动物贸易导致了新疆和内蒙古地区,以及内地的跨区域传播;细小病毒仅在羊来源的蜱虫中检测到,与中国河北地区的山羊血清中的细小病毒形成同一进化分支,我们推测蜱虫细小病毒在国内不同地区间可跨区域传播,在进化分析过程中,发现这种病毒与多种的细小病毒的同源性都不低于50％,提示细小病毒可能具有遗传稳定性;Tamdy病毒与来自阿塞拜疆、乌兹别克斯坦和美国的Tamdy病毒均具有极高的同源性,结果显示该病毒在内蒙古地区已经出现,并存在潜在流行的可能,有必要对Tamdy病毒进行进一步的监测;在本研究中,我们鉴定的白蛉病毒与来自新疆的亚洲璃眼蜱所携带的博乐蜱虱病毒形成同一个进化分支,与新型布尼亚病毒和Heartland virus病毒的同源性达到50％以上,该结果提示,我们发现的蜱虫白蛉病毒可能具有潜在的致病性,需要对其流行情况和致病性进行监测和研究.本研究为完善内蒙古部分地区蜱虫病毒的多样性和本底情况提供了重要的基础数据.     

Using zebrafish to study the complex genetics of glaucoma

The overall goal of this review is to highlight the power of zebrafish as a model system for studying complex diseases which involve multiple genetic loci. We are interested in identifying and characterizing genes implicated in the blinding condition of glaucoma. Glaucoma is a complex disease that often involves multiple genetic loci. Most disease causing and modifying genes for glaucoma remain unidentified. However, several genes that regulate various aspects of ocular development have been shown to associate with glaucoma. With zebrafish, forward and reverse genetic approaches can be combined in order to identify critical genetic interactions required for normal and pathological events in the development and maintenance of the eye.     

Immunoprophylaxis in fish by injection of mouse antibody genes

Antibodies are a crucial part of the body's specific defense against infectious diseases and have considerable potential as therapeutic and prophylactic agents in humans and animals. The development of recombinant single-chain antibodies allows a genetic application strategy for prevention of infectious diseases. To test this in a fish model, a gene construct encoding a neutralizing single-chain antibody to the fish-pathogenic rhabdovirus VHSV (viral hemorrhagic septicemia virus) was administered to rainbow trout by intramuscular injection of plasmid DNA. Circulating recombinant antibodies could later be detected in the fish, and protective immunity to the viral disease was established.     

Zebrafish as a model for hearing and deafness

The zebrafish is an especially attractive model for the study of the development and function of the vertebrate inner ear. It combines rapid and accessible embryogenesis with a host of genetic and genomic tools for systematic gene discovery and analysis. A large collection of mutations affecting development and function of the ear and a related sensory system, the lateral line, have been isolated; several of these have now been cloned, and at least five provide models for human deafness disorders. Disruption of multiple genes, using both forward and reverse genetic approaches, has established key players--both signaling molecules and autonomous factors--responsible for induction and specification of the otic placode. Vestibular and auditory defects have been detected in adult animals, making the zebrafish a useful system in which to tackle the genetic causes of late onset deafness and vestibular disease.     

Isolation of a lethal rhabdovirus from the cultured Chinese sucker Myxocyprinus asiaticus

A rhabdovirus was found to be associated with a lethal hemorrhagic disease in the cultured Chinese sucker Myxocyprinus asiaticus Bleeker. The rhabdovirus was amplified and isolated from the infected GCO (grass carp ovary) cells. In ultrathin sections of liver cells from the diseased fish, the virus particles exhibited the characteristic bacilliform morphology, and budded through vesicle membranes of the infected cells. The isolated rhabdovirus particles were found to have a bacilliform morphology with 2 rounded ends rather than a typical flat base. The virus particles were measured and ranged in size from 150 to 200 nm in length and 50 to 60 nm in diameter. Most other characteristics, including their size, extensive virus infectivity to fish cell lines, strong cytopathogenic effects, stability at high temperatures, vesicle formation in infected cells, structure protein electrophoretic patterns and the presence of an RNA genome, very closely resembled those of other fish rhabdoviruses. At present it is not known if this is a novel virus species or if it is an isolate of a known fish rhabdovirus. Until a confirmed identification can be made, we will temporarily refer to this virus as Chinese sucker rhabdovirus (CSRV).