人类乙型肝炎样病毒Pre—S1包膜蛋白的一个特定区域为乙肝病毒形成所必需

土拨鼠肝炎病毒（WHV）是一种哺乳类动物的肝炎病毒．这种病毒在结构和抗原怕与人类乙型肝炎病毒（HBV）非常相似．以往的研究报告指出,在一种称为鸭乙型肝炎病毒（DHBV）的Pre－S包膜蛋白中,含有一个特定区域．这一区域由天冬氨酸－天冬氨酸－脯氨酸－亮氨酸－亮氨酸（DDPLL）5个氨基酸残基所组成．已发现,这一区域在像DHBV这一类禽类乙肝病毒的病毒装配和分泌时所必需的（LenhoffR,SummersJ．JVirol,1994,68：4565～4571）．在WHV的Pre－S包胰蛋白中第201个氨基酸到第205个氨基酸所包含的顺序,甘氨酸－天冬氨酸－脯氨…     

Expression of the HTLV-III envelope gene by a recombinant vaccinia virus

The discovery that the aetiological agent of acquired immune deficiency syndrome (AIDS) is a retrovirus, referred to as human T-lymphotropic virus type III (HTLV-III) or lymphadenopathy-associated virus (LAV) (for review see ref. 1), has raised the possibility of developing a vaccine. In this regard, the envelope (env) proteins of murine retroviruses can induce protective immunity in mice. The HTLV-III env gene specifies a primary polypeptide of approximately 860 amino acids that is glycosylated to form a precursor of relative molecular mass (Mr) 160,000 (gp160), which gives rise to mature membrane-associated proteins of Mr 120,000 (gp120) and 41,000 (gp41). The HTLV-III env gene has been expressed in Escherichia coli and by simian virus 40 (SV40) vectors but formation of the authentic proteins has not been demonstrated. Here, we describe the expression of the complete env gene by a vaccinia virus vector. Evidence is presented that synthesis, glycosylation, processing and membrane transport of the env polypeptide occurred without other HTLV-III gene functions; the env protein was recognized by sera from unrelated AIDs patients; and a single vaccination with the infectious recombinant vaccinia virus induced antibodies to gp120 in mice.     

Hepatitis B polypeptide vaccine preparation in micelle form

The immunoprophylaxis of hepatitis B is hampered by the lack of a technique for growing hepatitis B virus (HBV) in tissue culture. Plasma from persistently infected individuals, one source of viral antigen, contains characteristic 22-nm spherical particles which share a common antigen (the hepatitis B surface antigen or HBsAg) with the outer envelope of the 42-nm double-shelled DNA virus. Highly purified inactivated 22-nm particles have been shown to be safe and to confer protective immunity against HBV in a recent large-scale clinical trial. We have already described the extraction from the particles of a complex of two proteins which are antigenic determinants of HBV--the polypeptide with molecular weight (MW) between 22,000 and 24,000 (called p23) and the glycosylated polypeptide (called gp28) with MW in the range 26,000--29,000 which is thought to be the glycosylated form of p23. We now report the preparation from this complex of water-soluble protein micelles which may be a suitable basis for a second-generation hepatitis B vaccine.     

Molecular cloning and sequencing of a human hepatitis delta (delta) virus RNA

Human hepatitis delta (delta) virus (HDV) is a form of defective virus, which infects humans only in the presence of a co-infecting hepatitis B virus (HBV). HDV superinfection in a chronic HBV carrier often results in severe chronic hepatitis and cirrhosis, whereas acute HDV and HBV co-infection is frequently associated with fulminant hepatitis. HDV consists of a 36-nm particle, which contains an envelope with HBV surface antigen, and a nucleocapsid containing the hepatitis delta-antigen (HDAg) and an RNA genome of 1.75 kilobases (kb). Recently, the genomic RNA from an HDV serially passaged in chimpanzees has been cloned and sequenced in a study which showed that the HDV RNA is a single-stranded circular molecule with properties similar to those of viroid or virusoid. However, it is not known whether serial passages in chimpanzees had altered the properties of human HDV. Here we report the cloning and sequencing of an HDV RNA isolated directly from a patient with acute delta-hepatitis. The sequence showed considerable divergence (11%) from that of the chimpanzee-adapted HDV. Five open reading frames (ORFs) of more than 100 amino acids in both genomic and anti-genomic sense were found. The largest ORF in antigenomic sense, which can code for 214 amino acids, may correspond to the HDAg.     

Improved immunogenicity of a peptide epitope after fusion to hepatitis B core protein

Synthetic vaccines for viral diseases can use defined regions of viral proteins as immunogens: the peptide sequence of amino acids 141-160 of the VP1 protein of foot and mouth disease virus (FMDV) elicits virus-neutralizing antibodies to protect guinea pigs, cattle and pigs either when coupled to a carrier protein or when administered in liposomes or in incomplete Freund's adjuvant. The immune response to these peptides is much lower than that to complete virus particles and the same sequence fused to the N terminus of beta-galactosidase did not produce a more potent immunogen than synthetic peptide alone. We report here an expression system for immunogenic epitopes linked to a carrier protein, hepatitis B core antigen, to form part of a virus-like complex which can present these epitopes to the immune system at high density. The immunogenicity of these structures approaches that of FMDV particles.     

An N-terminal peptide from p60src can direct myristylation and plasma membrane localization when fused to heterologous proteins

The src gene product, p60src, of Rous sarcoma virus (RSV) is a tyrosine-specific protein kinase which is associated with the plasma membrane of infected cells. Myristic acid is bound in an amide linkage to glycine 2 of p60src. Of the N-terminal 30 kilodaltons of p60src, only amino acids 1-14 are required for myristylation, and myristylation of p60src may be required for its membrane association, and for cell transformation. To test the hypothesis that the first 14 amino acids of p60src contain a recognition sequence for myristylation, we have fused the DNA sequence coding for these amino acids to either the fps gene of the F36 derivative of Fujinami sarcoma virus (FSV), or to the chimpanzee alpha-globin gene. We report here that although the fusion proteins were myristylated, the parental proteins were not, and unlike the non-myristylated F36 p91fps which was not bound to the plasma membrane, the myristylated fusion protein was bound, like p60src. We conclude that the first 14 amino acids of p60src contain a sequence which is sufficient for myristylation, and which may direct proteins to the plasma membrane.     

乙型肝炎病毒蛋白及COX-2在乙肝相关性肝细胞癌发展与转移中的作用机制

目的探讨乙型肝炎病毒蛋白及环氧合酶-2(COX-2)在乙肝相关性肝细胞癌发展与转移中的作用机制.方法取42例慢性乙肝患者行穿刺活检时乙型肝炎病毒ccc DNA为阳性乙肝相关性肝细胞癌组织;另取同期手术切除的11例ccc DNA为阴性的非乙型肝炎相关性肝癌组织.免疫组化法检测乙型肝炎病毒X蛋白、COX-2、CD34的表达水平,Werdner法计算微血管密度;分析上述因子与乙肝相关性肝细胞癌组织微血管生成的相关性.RT-PCR和Western blot检测人肝癌细胞系(HepG2)和稳定转染乙型肝炎病毒X蛋白(HepG2-X)细胞中COX-2mRNA和蛋白表达情况;ELISA法检测细胞上清液中PGE2表达水平和不同浓度COX-2抑制剂塞来昔布作用后PGE2水平.结果乙型肝炎病毒X蛋白阳性表达组织中COX-2阳性率明显高于乙型肝炎病毒X蛋白阴性表达组织和非乙型肝炎相关性肝癌组织(P0.01).乙型肝炎病毒X蛋白阳性表达组织中早期癌症微血管密度明显低于进展期癌症组织,乙型肝炎病毒X蛋白阴性表达组织中微血管密度明显低于阳性表达组织(P0.01);COX-2阳性表达组织中微血管密度明显高于COX-2阴性表达组织(P0.01);非乙型肝炎相关性肝癌组织中微血管密度明显低于乙型肝炎病毒X蛋白、COX-2阳性表达组织(P0.01),与乙型肝炎病毒X蛋白阴性表达组织和COX-2阴性表达组织之间差异无统计学意义(P0.05);乙型肝炎病毒X蛋白、COX-2在乙型肝炎相关性人肝细胞癌组织微血管生成呈正相关.HepG2-X细胞中COX-2 mRNA和蛋白表达水平明显高于空载体对照HepG2细胞,并且细胞培养上清液中PGE2水平明显增加;与HepG2细胞相比,塞来昔布对HepG2-X细胞分泌PGE2具有更强的抑制作用.结论乙型肝炎病毒X蛋白、COX-2在乙肝相关性肝细胞癌组织中高表达,促进了癌组织微血管生成;乙型肝炎病毒X蛋白可通过COX-2/PEG2信号通路促进了肝癌的发生和发展.     

Nucleotide sequence of the gene coding for the major protein of hepatitis B virus surface antigen.

DNA extracted from hepatitis B virus Dane particles has been cloned in bacteria using a plasmid vector. A full-length clone has been examined by restriction endonuclease analysis, and the nucleotide sequence of an 892-base pair fragment from cloned hepatitis B viral DNA encoding the surface antigen gene is reported. The amino acid sequence deduced from the DNA indicates that the surface antigens is a protein consisting of 226 amino acids and with a molecular weight of 25,398. The portion of the gene coding for this protein apparently contains no intervening sequences.     

Biosynthesis of hepatitis B virus surface antigen in Escherichia coli

Hepatitis B is a widespread viral disease. In the absence of cell cultures capable of propagating the virus (HBV) an efficient vaccine has been prepared from viral envelopes isolated from the plasma of chronic carriers. The major polypeptide of the envelope is one of molecular weight 25,000 which carries the surface antigen (HBsAg). Therefore, the biosynthesis of this polypeptide in Escherichia coli may offer an alternative procedure to produce HbsAg free from human proteins. Recently, the HBV genome has been cloned in E.coli. Determination of its primary structure allowed the localization of the gene (called gene S) coding for HBsAg and the synthesis of the core antigen in E.coli has been reported. We have constructed a derivative of bacteriophage lambda carrying a fusion between the beta-galactosidase gene (lacZ) and the HBsAg coding sequence (lambdalacHBs-1). Infection of E.coli with lambdalacHBs-1 leads to the biosynthesis of a polypeptide of molecular weitht 138,000 carrying antigenic determinants of HBV surface antigen.     

吉林地区病毒性肝炎分型分析

目的 了解吉林地区病毒性肝炎的型别分布及感染状况．方法 采用ELlSA法检测．结果 男性检出39例，女性检出21例，检出HAV23例，占38％；HBV25例，占42％，NCV6例，占10％；HVD未检出，HEV4例，占7％，HGV2例，占3％．乙型肝炎检出率最高，其次为甲型肝炎、丙型肝炎、戊型肝炎、庚型肝炎．丁型肝炎检出率为0．单纯感染56例；1例甲、丙、庚三重感染，1例为甲、乙二重感染．结论 甲、乙型肝炎仍为吉林地区人群感染的主要病原．     

Antibody production to the nucleocapsid and envelope of the hepatitis B virus primed by a single synthetic T cell site

The nucleocapsid (HBcAg) of the hepatitis B virus (HBV) can induce antibody responses via both a T-cell dependent and a T-cell independent pathway and is highly immunogenic during infection. We have examined the T-cell determinants of the antigen and find that HBcAg-specific helper T cells (TH) can help B cells produce antibody against envelope (HBsAg) antigens as well as HBcAg, even though these antigens are found on separate molecules. We have also been able to prime helper T cells with synthetic T-cell epitopes of HBcAg; helper cells primed with a single synthetic epitope can induce B cells to produce antibody that reacts with multiple HBsAg epitopes. One problem with the development of an HBV vaccine is that some vaccinees and patients do not respond to HBsAg directly; our results indicate that this problem can be circumvented using the response to HBcAg.     

Expression of AIDS virus envelope gene in recombinant vaccinia viruses

Acquired immune deficiency syndrome (AIDS) is an infectious disease characterized by severe impairment of the patient's cell-mediated immune system. Several lines of evidence have indicated that the aetiological agent of AIDS is a group of T-lymphotropic retroviruses, variously known as lymphadenopathy-associated virus (LAV), human T-lymphotropic virus type III (HTLV-III) and AIDS-associated retrovirus (ARV). Serological surveys have indicated that as many as one million people in the United States may have been infected by LAV/HTLV-III, and the spread of AIDS has become a global concern. The need for a better understanding of the viral immunology and for a vaccine against AIDS is self-evident. To this end, we have constructed recombinant vaccinia viruses containing the envelope (env) gene of LAV, and demonstrate here that cells infected with these viruses express immunoreactive proteins similar to those present on LAV virions. Experimental animals infected with these recombinant viruses elicited antibodies that specifically recognized LAV envelope proteins.     

Hepatitis B virus integration in a cyclin A gene in a hepatocellular carcinoma

Hepatitis B virus (HBV) DNA frequently integrates into the genome of human primary liver cancer cells, but the significance of this integration in liver carcinogenesis is still unclear. Here we report the cloning of a single HBV integration site in a human hepatocellular carcinoma at an early stage of development, and of its germline counterpart. The normal locus was found to be transcribed into two polyadenylated messenger RNA species of 1.8 and 2.7 kilobases. We have isolated a complementary DNA clone from a normal adult human liver cDNA library which has an open reading frame with a coding capacity for a protein of 432 amino acids and relative molecular mass 48,536. The strong homology of the C-terminal half of the protein to the A-type cyclins of clam and Drosophila identifies it as a human cyclin A. The cyclin A gene has several exons, and the HBV integration occurs within an intron. As cyclins are important in the control of cell division, the disruption of a cyclin A gene by viral insertion might contribute to tumorigenesis.     

Mimicking the alloantigenicity of proteins with chemically synthesized peptides differing in single amino acids

Recent studies have shown that short chemically synthesized peptides very often induce antibodies which react with the cognate sequence in the intact folded protein. Since such antibodies react with known regions of proteins, they are of predetermined specificity and offer a precision not previously possible with immunological probes. A basic concept emerging from the use of such antibodies in viral systems is that the differential immunogenicity of closely related proteins can be mimicked by short peptides which span the regions of sequence variation. To generalize this concept, we have studied the two Thy-1 proteins which vary by only a single amino acid. Chemically synthesized peptides differing in only one out of 19 amino acids were able to induce allospecific antisera. Thus, single amino acid changes have similar effects on the immunogenicity of proteins and small peptides, even though the latter are free from constraints provided by neighbouring structures in the tertiary configuration of the intact folded proteins.     

乙肝病毒感染数量的一个数学模型

乙型肝炎是由乙型肝炎病毒(HBV)引起的肝病,该病毒干扰肝功能并造成病理损害.一小部分受感染者无法消灭该病毒而成为慢性感染,进而面临极高的死于肝硬化和肝癌的危险.乙型肝炎病毒通过与受感染者的血液或体液接触传播,这与人类免疫缺陷病毒(艾滋病毒)的方式相同.但是,乙型肝炎病毒的感染性比艾滋病毒高50至100倍.接种乙型肝炎疫苗是预防乙型肝炎的主要方法.如何有效防控乙肝的传染,不只是政府的事,也是每个国民应关注的问题.文章建立一个乙肝病毒传染的数学模型,并对模型进行实证分析;同时,对乙肝病毒的传染也做了一个预测.     

Immune sera recognize on erythrocytes Plasmodium falciparum antigen composed of repeated amino acid sequences

Protective immune responses against the asexual stages of the human malaria parasite, Plasmodium falciparum, are most probably directed against exposed antigenic determinants on the surface of the free merozoite or the infected red blood cell, and therefore antigens in these locations are candidates for testing as components of a defined molecular vaccine. To facilitate the search for such antigens, we recently developed a method for the expression of P. falciparum proteins in Escherichia coli as fused polypeptides. Many clones producing antigens were detected by screening with immune human sera. We show here that antibodies against the fused polypeptide expressed by one such clone react with a P. falciparum protein that is synthesized late in schizogony and is later present on the surface of the ring-infected erythrocyte. The protein is composed of repeating subunits of 8, 4 and 3 amino acids and is present in all isolates of P. falciparum examined.