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传染性法氏囊病病毒的病毒蛋白3在原核和真核表达系统中表达后不能保护鸡抵抗该病。

Failure of viral protein 3 of infectious bursal disease virus produced in prokaryotic and eukaryotic expression systems to protect chickens against the disease.

作者信息

Pitcovski J, Levi B Z, Maray T, Di-Castro D, Safadi A, Krispel S, Azriel A, Gutter B, Michael A

机构信息

MIGAL, South Industrial Area, Kiryat Shmona, Israel.

出版信息

Avian Dis. 1999 Jan-Mar;43(1):8-15.

Abstract

In recent years, infectious bursal disease virus (IBDV) has become a serious economic problem as a result of the emergence of new and very virulent strains. Most of the antibodies produced against IBDV are for the structural proteins viral protein (VP) 2 (VP2) and VP3. The purpose of this study was to test the potential of recombinant VP3 to induce protective antibodies. The gene for VP3 was isolated from a virulent strain of the virus and cloned into prokaryotic (Escherichia coli) and eukaryotic (baculovirus) expression systems. The protein expressed by both systems was of the expected size (32 kD) and was detected by anti-IBDV antibodies. Following partial purification, the polypeptides were injected into intact birds and induced the production of high levels of anti-IBDV antibodies, as detected by immunoblot and enzyme-linked immunosorbent assay tests. These antibodies did not prevent changes in the bursa and mortality when birds were challenged with a virulent IBDV strain after vaccination with the recombinant VP3. The results show that VP3 polypeptide cannot be used as a subunit vaccine against IBDV and raise questions concerning the nature of the neutralizing epitope on this structural protein.

摘要

近年来,由于新的超强毒株的出现,传染性法氏囊病病毒(IBDV)已成为一个严重的经济问题。针对IBDV产生的大多数抗体是针对结构蛋白病毒蛋白(VP)2(VP2)和VP3的。本研究的目的是测试重组VP3诱导保护性抗体的潜力。从该病毒的一个强毒株中分离出VP3基因,并将其克隆到原核(大肠杆菌)和真核(杆状病毒)表达系统中。两个系统表达的蛋白大小均符合预期(32 kD),且能被抗IBDV抗体检测到。经过部分纯化后,将这些多肽注射到完整的禽类体内,并通过免疫印迹和酶联免疫吸附试验检测到诱导产生了高水平的抗IBDV抗体。在用重组VP3疫苗接种后,当禽类受到强毒IBDV毒株攻击时,这些抗体并不能阻止法氏囊的变化和死亡。结果表明,VP3多肽不能用作抗IBDV的亚单位疫苗,并引发了关于该结构蛋白上中和表位性质的问题。

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