GENOME OF THE CELL FUSING AGENT
细胞融合剂的基因组
基本信息
- 批准号:3140167
- 负责人:
- 金额:$ 11.74万
- 依托单位:
- 依托单位国家:美国
- 项目类别:
- 财政年份:1988
- 资助国家:美国
- 起止时间:1988-08-01 至 1993-07-31
- 项目状态:已结题
- 来源:
- 关键词:Alphavirus Culicidae Flaviviridae Herpesviridae disease RNA methylation RNA virus cell fusion disease vectors gel electrophoresis genetic mapping genetic translation genome interfering virus laboratory mouse methyltransferase molecular cloning nucleic acid sequence open reading frames protein sequence recombinant DNA virus RNA virus envelope virus genetics virus protein virus replication
项目摘要
About 12 years ago we discovered a new virus in our laboratory.
The virus was present in the culture medium of an Aedes aegypti
cell lie and was recognized because it caused fusion of Aedes
albopictus cells. We called it CFA for cell fusing agent. We
showed, at that time, that CFA was a 50 nm spherical, enveloped
virus with a (+) strand RNA genome, that it replicated in the
cytoplasm, and that it had three structural proteins. Although in
these respects CFA resembled the togaviruses and flaviviruses, it
shown no serological cross reaction with viruses in either of these
two families. At present, the taxonomic status of CFA still
remains unsettled.
We propose now to extend our studies of CFA. There are two
compelling reasons for undertaking these studies now. Within the
past 6 months we have isolated by endpoint dilution, clones of CFA
which replicate more quickly and produce yields 50-100 fold higher
than our original strain. This will greatly facilitate biochemical
studies. Secondly, since our original work was done, the field of
recombinant DNA technology has emerged making possible new
approaches to the study of viruses.
In this proposal we describe experimental approaches which will
help us learn more about how CFA replicates and about some of its
biological properties. A major effort will be directed to the
cloning and sequencing of the CFA genome. The information obtained
will enable us to determine the number of open reading frames, to
deduce the amino acid sequences of the viral proteins, and to see
if there is any homology between CFA RNA and other viral RNAs. In
direct studies on the CFA viral RNA we shall determine the
nucleotide sequence of the 3' terminus of the RNA, in the process
learning whether the RNA is polyadenylated, and we shall
characterize the cap structure at the 5' terminus of the RNA. The
CFA proteins will be sequenced at their N-termini so that their
coding sequences can be aligned on the viral genome. Mutants of
CFA will be selected, as we have done with Sindbis virus, which
code for altered RNA capping and methylating enzymes. These will
eventually be used for identifying the genes which code for these
enzymes. We shall investigate in more detail the host range of
CFA, testing its ability to replicate in other mosquito cell lines,
in Drosophila and lepidopteran lines, and in selected vertebrate
cells including a fathead minnow line. We shall test whether CFA
can interfere with alpha and flaviviruses. Finally, we shall
screen mosquitoes in New Jersey for viruses which resemble CFA.
From these studies we shall 1) obtain a better understanding of how
CFA replicates, 2) help settle the taxonomic status of CFA, and 3)
gain insights into the evolution of small enveloped RNA viruses,
including the arthropod-borne viruses which cause disease in man.
大约12年前,我们在实验室发现了一种新病毒。
该病毒存在于埃及伊蚊的培养液中。
细胞撒谎,因为它导致伊蚊的融合而被识别
白纹伊蚊细胞。我们称它为细胞融合剂的CFA。我们
当时显示,CFA是一个50纳米的球形,被包裹
带有(+)链RNA基因组的病毒,它在
细胞质,它有三种结构蛋白。虽然在
在这些方面,CFA类似于托加病毒和黄病毒,它
在这两种病毒中都没有表现出与病毒的血清学交叉反应
两个家庭。目前,CFA的分类地位仍然是
仍然悬而未决。
我们现在建议扩大对终审法院的研究。有两个
现在进行这些研究的令人信服的理由。在
在过去的6个月里,我们通过终点稀释分离了CFA的克隆
它们的复制速度更快,产量提高50-100倍
而不是我们最初的菌株。这将极大地促进生化
学习。第二,由于我们最初的工作已经完成,所以领域
重组DNA技术的出现使新的
研究病毒的方法。
在这份提案中,我们描述了实验方法,它将
帮助我们更多地了解CFA是如何复制的,以及一些
生物学特性。将作出重大努力,以
CFA基因组的克隆和测序。所获得的信息
将使我们能够确定开放阅读框的数量,以
推导出病毒蛋白的氨基酸序列,并观察到
如果CFA RNA与其他病毒RNA之间有任何同源性。在……里面
对CFA病毒RNA的直接研究我们将确定
RNA3‘末端的核苷酸序列,在这个过程中
了解RNA是否是多腺化的,我们将
描述RNA 5‘末端的帽子结构。这个
CFA蛋白将在其N-末端进行测序,以便其
编码序列可以在病毒基因组上进行比对。突变体
将选择CFA,就像我们对Sindbis病毒所做的那样,它
改变的RNA封顶和甲基化酶的代码。这些遗嘱
最终被用来识别编码这些基因的基因
酵素。我们将更详细地调查寄主范围
CFA正在测试其在其他蚊子细胞系中复制的能力,
在果蝇和鳞翅目昆虫品系中,以及在选定的脊椎动物中
包括一条愚人鱼生产线在内的牢房。我们将测试终审法院是否
可以干扰阿尔法病毒和黄病毒。最后,我们将
在新泽西州对蚊子进行类似CFA的病毒筛查。
从这些研究中,我们将更好地了解
CFA复制,2)帮助确定CFA的分类地位,3)
洞察小包膜RNA病毒的进化,
包括节肢动物传播的病毒,这种病毒会导致人类患病。
项目成果
期刊论文数量(2)
专著数量(0)
科研奖励数量(0)
会议论文数量(0)
专利数量(0)
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VICTOR STOLLAR其他文献
VICTOR STOLLAR的其他文献
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{{ truncateString('VICTOR STOLLAR', 18)}}的其他基金
Regulation of Sindbis Virus Subgenomic RNA Synthesis
辛德毕斯病毒亚基因组 RNA 合成的调控
- 批准号:
8080585 - 财政年份:2010
- 资助金额:
$ 11.74万 - 项目类别:
Regulation of Sindbis Virus Subgenomic RNA Synthesis
辛德毕斯病毒亚基因组 RNA 合成的调控
- 批准号:
7228863 - 财政年份:2006
- 资助金额:
$ 11.74万 - 项目类别:
Regulation of Sindbis Virus Subgenomic RNA Synthesis
辛德比斯病毒亚基因组 RNA 合成的调控
- 批准号:
7132599 - 财政年份:2006
- 资助金额:
$ 11.74万 - 项目类别:
Regulation of Sindbis Virus Subgenomic RNA Synthesis
辛德比斯病毒亚基因组 RNA 合成的调控
- 批准号:
7417874 - 财政年份:2006
- 资助金额:
$ 11.74万 - 项目类别:
Nucleotide Pools and the Replication of Sindbis Virus
核苷酸库和辛德比斯病毒的复制
- 批准号:
6534319 - 财政年份:2001
- 资助金额:
$ 11.74万 - 项目类别:
Nucleotide Pools and the Replication of Sindbis Virus
核苷酸池和辛德比斯病毒的复制
- 批准号:
6619848 - 财政年份:2001
- 资助金额:
$ 11.74万 - 项目类别:
Nucleotide Pools and the Replication of Sindbis Virus
核苷酸库和辛德比斯病毒的复制
- 批准号:
6437968 - 财政年份:2001
- 资助金额:
$ 11.74万 - 项目类别:
相似国自然基金
蚊科CULICIDAE专家系统
- 批准号:38870106
- 批准年份:1988
- 资助金额:4.0 万元
- 项目类别:面上项目
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