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利用肽展示文库探究猫白血病病毒包膜蛋白受体靶向结构域中的序列变异。

Probing sequence variation in the receptor-targeting domain of feline leukemia virus envelope proteins with peptide display libraries.

作者信息

Bupp Keith, Sarangi Anindita, Roth Monica J

机构信息

Department of Biochemistry, Robert Wood Johnson Medical School, University of Medicine and Dentistry of New Jersey, 675 Hoes Lane, Piscataway, NJ 08854, USA.

出版信息

J Virol. 2005 Feb;79(3):1463-9. doi: 10.1128/JVI.79.3.1463-1469.2005.

Abstract

Determinants of cellular tropism and receptor targeting lie within a short peptide in the Vr1 region of the envelope (Env) proteins of feline leukemia virus (FeLV) subgroups A and C. Libraries of FeLV Env proteins with random amino acid substitutions in the peptide were screened for their ability to deliver a marker gene to D17 and AH927 cells. Screening on D17 canine cells yielded D17-specific Env proteins that used the FeLV-C receptor. Screening on AH927 cells yielded Env proteins with a broader host range, with maximal titers on AH927 cells and similar or lower titers on other cells. These Env proteins used an unidentified non-FeLV receptor for entry. The A5 isolate obtained from the AH927 screen was readily concentrated to yield titers of 10(5) on human PC-3 prostate tumor cells. The sequence divergence observed among targeting peptides of library-selected Env proteins was greater than that found in parental FeLV isolates. Substitution analyses of a conserved R in the middle of the targeting peptide held constant during screening indicated that maximal titers were obtained only when R was present in both a D17 selected isolate and an AH927 selected isolate. The ability to isolate Env proteins with unique tropisms dependent on the cells on which the library is screened has direct implications for targeting gene delivery vectors.

摘要

猫白血病病毒(FeLV)A 亚群和 C 亚群包膜(Env)蛋白的 Vr1 区域中的一段短肽决定了细胞嗜性和受体靶向。对该肽段具有随机氨基酸替换的 FeLV Env 蛋白文库进行筛选,以检测其将标记基因传递至 D17 和 AH927 细胞的能力。在 D17 犬类细胞上进行筛选,得到了使用 FeLV-C 受体的 D17 特异性 Env 蛋白。在 AH927 细胞上进行筛选,得到了宿主范围更广的 Env 蛋白,其在 AH927 细胞上的滴度最高,而在其他细胞上的滴度相似或更低。这些 Env 蛋白利用一种未鉴定的非 FeLV 受体进入细胞。从 AH927 筛选中获得的 A5 分离株很容易浓缩,在人 PC-3 前列腺肿瘤细胞上产生的滴度为 10(5)。在文库选择的 Env 蛋白的靶向肽中观察到的序列差异大于在亲本 FeLV 分离株中发现的差异。在筛选过程中保持恒定的靶向肽中间保守的 R 的替换分析表明,只有当 R 同时存在于 D17 选择的分离株和 AH927 选择的分离株中时,才能获得最高滴度。根据筛选文库所用的细胞分离具有独特嗜性的 Env 蛋白的能力,对靶向基因传递载体具有直接影响。

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