Ketha Krishna Mohan V, Atreya Chintamani D
Section of Cell Biology, Laboratory of Cellular Hematology, Division of Hematology, Office of Blood Research and Review, Center for Biologics Evaluation and Research (F,D,A,) Bethesda, MD 20892, USA.
BMC Cell Biol. 2008 Apr 28;9:22. doi: 10.1186/1471-2121-9-22.
Two nuclear localization sequences (NLS) in influenza A virus nucleoprotein (NP) have been demonstrated to be critical for nuclear import of NP and viral ribonucleoprotein complexes. However, a deletion mutant lacking these two signals was still able to localize to the nucleus suggesting the presence of yet another (a third) potential NLS in the NP protein. In order to identify the nature of this potential NLS signal in the NP of a WS/33L influenza virus A strain, we utilized the tools of bioinformatics coupled with functional experimental analyses in the present study.
Comparison of the deduced aa sequence of NP of WS/33L strain with the published WS/33 NP sequences revealed that a single amino acid (aa) change (Met to Arg) at position 105 results in converting the flanking regions (between aa position 90-121, a 32-residue stretch) into two classical overlapping bipartite NLS (obpNLS). GenBank search revealed that 9 out of 500 published NP sequences contain a similar Arg at position 105 (instead of Met) with a 100% homology to the obpNLS region. Various NP-green fluorescent protein (GFP) fusion constructs with and without the signal (obpNLS-Arg105) were utilized to understand the functional nature of this signal. We analyzed the transport competency of the expressed chimeric proteins in terms of their cellular localization by confocal immunofluorescence assay. Our analysis revealed that all NP-GFP constructs containing the wild-type (R105) sequence localized predominantly to the nucleus. Constructs lacking the obpNLS or constructs with reverse mutation (R105 to M105) on the other hand exhibited predominant cytoplasmic localization pattern. Interestingly, when the 32 aa obpNLS was fused with an unrelated viral protein (rotavirus NSP6) that has been known to be cytoplasmic protein, the chimeric protein (obpNLS-NSP6) was efficiently transported into the nucleus, indicating an efficient nuclear transport function of the 32-residue obpNLS in the NP of WS/33L strain of influenza A virus.
This report while not only establishing a new NLS in the influenza A virus strain, it also reinforces the idea that proper application of bioinformatics-coupled experimental analysis serves as a powerful tool in identifying new functional signals in proteins of interest.
甲型流感病毒核蛋白(NP)中的两个核定位序列(NLS)已被证明对NP和病毒核糖核蛋白复合体的核输入至关重要。然而,一个缺失这两个信号的缺失突变体仍能够定位于细胞核,这表明NP蛋白中还存在另一个(第三个)潜在的NLS。为了确定WS/33L甲型流感病毒株NP中这个潜在NLS信号的性质,在本研究中我们利用了生物信息学工具并结合功能实验分析。
将WS/33L株NP的推导氨基酸序列与已发表的WS/33 NP序列进行比较,发现在第105位的单个氨基酸变化(Met变为Arg)导致侧翼区域(在氨基酸位置90 - 121之间,一个32个残基的片段)转变为两个经典的重叠双分型NLS(obpNLS)。GenBank搜索显示,在500个已发表的NP序列中,有9个在第105位含有类似的Arg(而非Met),与obpNLS区域具有100%的同源性。利用各种带有和不带有该信号(obpNLS-Arg105)的NP-绿色荧光蛋白(GFP)融合构建体来了解该信号的功能性质。我们通过共聚焦免疫荧光分析,根据表达的嵌合蛋白的细胞定位来分析其转运能力。我们的分析表明,所有含有野生型(R105)序列的NP-GFP构建体主要定位于细胞核。另一方面,缺乏obpNLS的构建体或具有反向突变(R105变为M105)的构建体则表现出主要的细胞质定位模式。有趣的是,当32个氨基酸的obpNLS与一种已知为细胞质蛋白的无关病毒蛋白(轮状病毒NSP6)融合时,嵌合蛋白(obpNLS-NSP6)被有效地转运到细胞核中,这表明甲型流感病毒WS/33L株NP中32个残基的obpNLS具有有效的核转运功能。
本报告不仅在甲型流感病毒株中确定了一个新的NLS,还强化了这样一种观点,即生物信息学与实验分析的恰当应用是识别目标蛋白中新功能信号的有力工具。
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