66 results on '"G. Herrler"'
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2. Leukozytenpopulationen und Zytokinexpression in der Lunge im Verlauf der Hundestaupevirus-Infektion
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E Chludzinski, J Klemens, M Ciurkiewicz, D-L Shin, G Herrler, and A Beineke
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- 2022
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3. Sialic Acid Binding Activity of Transmissible Gastroenteritis Coronavirus Affects Sedimentation Behavior of Virions and Solubilized Glycoproteins
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G. Herrler and Christine Krempl
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Swine ,viruses ,Immunology ,Transmissible gastroenteritis coronavirus ,Neuraminidase ,Sialic acid binding ,medicine.disease_cause ,Microbiology ,chemistry.chemical_compound ,Viral Proteins ,Glucosides ,Virology ,medicine ,Centrifugation, Density Gradient ,Animals ,Binding site ,Coronavirus ,chemistry.chemical_classification ,biology ,Structure and Assembly ,Transmissible gastroenteritis virus ,Virion ,Viral membrane ,biology.organism_classification ,Molecular biology ,N-Acetylneuraminic Acid ,Sialic acid ,Amino acid ,Microscopy, Electron ,Biochemistry ,chemistry ,Solubility ,Insect Science ,biology.protein - Abstract
Transmissible gastroenteritis coronavirus (TGEV) is a prototype enteropathogenic coronavirus that causes diarrhea in pigs of all ages. While adult animals usually recover, newborn piglets generally die from the intestinal infection (14). TGEV is an enveloped virus with three proteins inserted into the viral membrane: S (220 kDa), M (29 to 36 kDa), and E (10 kDa), a minor protein. The S protein plays a key role in the initial stage of infection. It mediates binding of the virus to the cell surface and the subsequent fusion between the viral and cellular membranes. Two binding activities have been assigned to the S protein. Binding to porcine aminopeptidase N, a cellular receptor for TGEV, is a prerequisite for infection of cells (5). A second binding activity enables TGEV to recognize sialic acid residues and attach to sialoglycoconjugates (18). As a consequence of the latter binding activity, TGEV can agglutinate erythrocytes (11, 12). The binding site for aminopeptidase N and the binding site for sialic acid are located on different portions of the S protein (18). Recent studies with mutants of TGEV indicated that a short stretch of amino acids (145 to 209) is important for the recognition of sialic acids (8). Some of the mutants had been selected for resistance to a monoclonal antibody. Interestingly, the point mutations that were responsible for the lack of antibody reactivity also resulted in the concomitant loss of both hemagglutinating activity and enteropathogenicity (8). These results indicated not only that the respective amino acids are located at or close to the sialic acid binding site but also that the sialic acid binding activity is correlated with the enteropathogenicity of TGEV. Other factors may also be required to render TGEV enteropathogenic, but they have not been identified in terms of a molecular interaction. The importance of the sialic acid binding activity for enteropathogenicity is supported by data reported for porcine respiratory coronavirus (PRCoV), which is closely related to TGEV. This virus replicates with high efficiency in the respiratory tract but with very low efficiency in the gut (4). Like the mutants mentioned above, PRCoV has no hemagglutinating activity (18). In the case of PRCoV, the lack of a sialic acid binding activity is explained by a large deletion in the S gene that results in a truncated spike protein (15, 16). The point mutations that resulted in the loss of hemagglutinating activity and enteropathogenicity are located in that portion of the S protein that is present in the TGEV S protein but absent from the PRCoV S protein. Here we report that the ability of TGEV to attach to sialoglycoconjugates affects the physical state of virus particles. TGEV with a functional sialic acid binding activity was recovered from sucrose gradients at higher densities than PRCoV or mutants of TGEV with a defect in the sialic acid binding site. The difference in sedimentation behavior was also observed with solubilized S protein. It was abolished after neuraminidase treatment of virions, suggesting that bound sialoglycoproteins are responsible for the different sedimentation characteristics. (Part of this work was done by C.K. in partial fullfilment of the requirements for the Dr. rerum physiologicarum degree at Philipps-Universitat Marburg, Marburg, Germany.)
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- 2001
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4. Characterization of the sialic acid binding activity of transmissible gastroenteritis coronavirus by analysis of haemagglutination-deficient mutants
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Gert Zimmer, M. L. Ballesteros, Hans-Dieter Klenk, Luis Enjuanes, C. Krempl, and G. Herrler
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Swine ,Detergents ,Mutant ,Transmissible gastroenteritis coronavirus ,Hemagglutinins, Viral ,Sialic acid binding ,Antibodies, Viral ,Sialidase ,Microbiology ,Virus ,Viral Proteins ,chemistry.chemical_compound ,Glucosides ,Animals ,Point Mutation ,chemistry.chemical_classification ,biology ,Gastroenteritis, Transmissible, of Swine ,Hemagglutination ,Transmissible gastroenteritis virus ,Mucins ,Antibodies, Monoclonal ,Drug Resistance, Microbial ,biology.organism_classification ,Virology ,Molecular biology ,N-Acetylneuraminic Acid ,Amino acid ,Sialic acid ,chemistry ,Biochemistry ,biology.protein ,Neuraminidase - Abstract
Transmissible gastroenteritis coronavirus (TGEV) agglutinates erythrocytes of several species by virtue of sialic acid binding activity of the surface protein S. We have isolated and characterized five haemagglutination-defective (HAD) mutants. In contrast to the parental virus, the mutants were unable to bind to porcine submandibulary mucin, a substrate rich in sialic acid. Each of the mutants was found to contain a single point mutation in the S protein (Cys155Phe, Met195Val, Arg196Ser, Asp208Asn or Leu209Pro), indicating that these amino acids are affecting the sialic acid binding site. In four of the HAD mutants a nearby antigenic site is affected in addition to the sialic acid binding site, as indicated by reactivity with monoclonal antibodies. The parental virus was found to have an increased resistance to the detergent octylglucoside compared to the HAD mutants. This effect depended on cellular sialoglycoconjugates bound to the virion. If the binding of sialylated macromolecules was prevented by neuraminidase treatment, the parental virus was as sensitive to octylglucoside as were the HAD mutants. We discuss the possibility that the sialic acid binding activity helps TGEV to resist detergent-like substances encountered during the gastrointestinal passage and thus facilitates the infection of the intestinal epithelium. An alternative function of the sialic acid binding activity – accessory binding to intestinal tissues – is also discussed.
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- 2000
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5. Importance of the Carboxyl-terminal FTSL Motif of Membrane Cofactor Protein for Basolateral Sorting and Endocytosis
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Andrea Maisner, G. Herrler, and Meike Teuchert
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CD46 ,media_common.quotation_subject ,Cell Biology ,Apical membrane ,Biology ,Endocytosis ,Biochemistry ,Fusion protein ,Cell biology ,Tyrosine ,Sequence motif ,Internalization ,Molecular Biology ,media_common ,Epithelial polarity - Abstract
Membrane cofactor protein (MCP), a widely distributed complement regulatory protein, is expressed on the basolateral surface of polarized epithelial cells, and it is not endocytosed. The carboxyl-terminal tetrapeptide (FTSL) is required for polarized surface expression. The ability of this tetrapeptide to serve as an autonomous sorting signal has been analyzed by adding this sequence motif to the C terminus of an apical membrane protein, the influenza A virus hemagglutinin (HA). The recombinant protein HA-FTSL retained the apical localization of the parental HA protein. Substitution of the complete cytoplasmic tail of MCP for the cytoplasmic tail of HA resulted in the targeting of the chimeric protein (HA/MCP) to the basolateral surface suggesting that the carboxyl-terminal FTSL motif is a weak sorting signal that requires additional targeting information from the membrane-proximal part of the cytoplasmic tail of MCP for redirecting an apical protein to the basolateral membrane domain. In contrast to the native HA, the HA-FTSL protein was subject to endocytosis. The basolateral HA/MCP was also found to be internalized and thus differed from the basolateral MCP. This result suggests that the carboxyl-terminal FTSL motif serves as an internalization signal and that in native MCP sorting information outside the cytoplasmic tail counteracts this endocytosis signal. Substitution of a tyrosine for the phenylalanine dramatically increased the internalization with most of the HA-YTSL protein being present intracellularly. Our results are consistent with the view that the interplay of multiple sorting signals and the modification of a well known targeting signal (YTSL) by amino acid exchange (FTSL) determine the constitutive expression of MCP on the basolateral surface of polarized epithelial cells.
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- 1999
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6. Membrane Cofactor Protein (CD46) Is a Basolateral Protein That Is Not Endocytosed
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Douglas M. Lublin, John P. Atkinson, M K Liszewski, Andrea Maisner, G. Herrler, and Gert Zimmer
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Alanine ,chemistry.chemical_classification ,Tetrapeptide ,CD46 ,Phenylalanine ,Cell Biology ,Biology ,Endocytosis ,Biochemistry ,Amino acid ,chemistry ,Tyrosine ,Molecular Biology ,Peptide sequence - Abstract
Membrane cofactor protein (MCP) is a widely distributed complement regulatory protein that is expressed on the basolateral surface of polarized epithelial cells. The basolateral targeting of the BC1 isoform of MCP was analyzed by generating deletion mutants and point mutants within the cytoplasmic tail of 16 amino acids. A sequence of four amino acids, FTSL, was found to be indispensable for the basolateral transport of MCP. This tetrapeptide has two unique features compared with the targeting motifs of other basolateral proteins: (i) it contains a phenylalanine rather than a tyrosine at position 1; (ii) it is located at the very COOH-terminal end. Replacement of the phenylalanine or the leucine by an alanine resulted in a nonpolarized delivery to the cell surface. On the other hand, substitution of a tyrosine for the phenylalanine did not affect the basolateral transport of MCP. The latter mutant, however, was efficiently internalized, whereas the wild type protein was not subject to endocytosis. Our results indicate that the targeting signal YXX-large aliphatic that is involved in various sorting events has been modulated in MCP in such a way that it allows basolateral transport but not endocytosis.
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- 1997
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7. Transfer of an Esterase-Resistant Receptor Analog to the Surface of Influenza C Virions Results in Reduced Infectivity Due to Aggregate Formation
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Katja Höfling, G. Herrler, Hans-Dieter Klenk, and Reinhard Brossmer
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Influenzavirus C ,viruses ,Molecular Sequence Data ,Chick Embryo ,Esterase ,Virus ,Cell Line ,Viral Proteins ,chemistry.chemical_compound ,Dogs ,Virology ,Animals ,Humans ,chemistry.chemical_classification ,Infectivity ,biology ,Hemagglutination ,Acetylesterase ,Sialic acid ,Enzyme ,Carbohydrate Sequence ,chemistry ,Sialic Acids ,biology.protein ,Receptors, Virus ,Influenza C Virus ,Neuraminidase - Abstract
A synthetic sialic acid, N -acetyl-9-thioacetamidoneuraminic acid (9-ThioAcNeu5Ac), is recognized by influenza C virus as a receptor determinant but—in contrast to the natural receptor determinant, N -acetyl-9- O -acetylneuraminic acid—is resistant to inactivation by the viral acetylesterase. This sialic acid analog was used to analyze the importance of the receptor-destroying enzyme of influenza C virus in keeping the viral surface free of receptor determinants. Enzymatic transfer of 9-ThioAcNeu5Ac to the surface of influenza C virions resulted in the loss of the hemagglutinating activity. The ability to agglutinate erythrocytes was restored when the synthetic sialic acid was released from the viral surface by neuraminidase treatment. Infectivity of influenza C virus containing surface-bound 9-ThioAcNeu5Ac was reduced about 20-fold. Sedimentation analysis as well as electron microscopy indicated that virions resialylated with the esterase-resistant sialic acid analog formed virus aggregates. These results indicate that the receptor-destroying enzyme of influenza C virus is required to avoid the presence of receptor determinants on the virion surface and thus to prevent aggregate formation and a reduction of the infectious titer.
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- 1996
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8. The catalytic triad of the influenza C virus glycoprotein HEF esterase: characterization by site-directed mutagenesis and functional analysis
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Hans-Dieter Klenk, S. Pleschka, and G. Herrler
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Influenzavirus C ,Isoflurophate ,Recombinant Fusion Proteins ,Molecular Sequence Data ,Hemagglutinins, Viral ,Hemagglutinin Glycoproteins, Influenza Virus ,Biology ,Esterase ,Cell Line ,Serine ,Viral Proteins ,Dogs ,Virology ,Catalytic triad ,Animals ,Histidine ,Amino Acid Sequence ,Enzyme Inhibitors ,Site-directed mutagenesis ,chemistry.chemical_classification ,Aspartic Acid ,Binding Sites ,Expression vector ,Serine Endopeptidases ,NF-kappa B ,Molecular biology ,Amino acid ,chemistry ,Biochemistry ,Mutagenesis, Site-Directed ,Sialic Acids ,Acetylesterase ,Influenza C Virus ,Carboxylic Ester Hydrolases ,Viral Fusion Proteins - Abstract
Influenza C virus is able to inactivate its own cellular receptors by virtue of a sialate 9-O-acetylesterase that releases the acetyl residue at position C-9 of N-accetyl-9-O-acetylneuraminic acid (Neu5,9Ac2). The receptor-destroying enzyme activity is a function of the surface glycoprotein HEF and this esterase belongs to the class of serine hydrolases. In their active site, these enzymes contain a catalytic triad made up of a serine, a histidine and an aspartic acid residue. Sequence comparison with other serine esterases has indicated that, in addition to serine-71 (S71), the amino acids histidine-368 or -369 (H368/369) and aspartic acid 261 (D261) are the most likely candidates to form the catalytic triad of the influenza C virus glycoprotein. By site-directed mutagenesis, mutants were generated in which alanine substituted for either of these amino acids. Using a phagemid expression vector, pSP1D-HEF the HEF gene was expressed in both COS 7 and MDCK I cells. The glycoprotein was obtained in a functional form only in the latter cells, as indicated by its transport to the cell surface and measurable enzyme activity. The low level of expression could be increased by stimulating the NF-κB-binding activity of the cytomegalovirus immediate-early promoter/enhancer element of the vector. The esterase activity of the mutant proteins was compared with that of the wild-type glycoprotein. With Neu5,9Ac2 as the substrate, the esterase specific activities of the S71/A mutant and the H368,369/A mutant were reduced by more than 90%. In the case of the D261/A mutant the specific activity was reduced by 64%. From this data we conclude that S71, H368/369 and D261 are likely to represent the catalytic triad of the influenza C virus glycoprotein HEF. In addition, N280 is proposed to stabilize the oxyanion of the presumptive transition state intermediate formed by the enzyme-substrate complex.
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- 1995
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9. A synthetic sialic acid analogue is recognized by influenza C virus as a receptor determinant but is resistant to the receptor-destroying enzyme
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H.J. Gross, G Milks, A Imhof, R Brossmer, James C. Paulson, and G. Herrler
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chemistry.chemical_classification ,biology ,Sialyltransferase ,Orthomyxoviridae ,Biological activity ,Cell Biology ,biology.organism_classification ,Biochemistry ,Virus ,Sialic acid ,carbohydrates (lipids) ,chemistry.chemical_compound ,Enzyme ,chemistry ,biology.protein ,Influenza C Virus ,Receptor ,Molecular Biology - Abstract
Synthetic sialic acid analogues varying in the substitutents at position C-9 were analyzed for their ability to replace the natural receptor determinant for influenza C virus, N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2). By incubation of erythrocytes with sialyltransferase and the CMP-activated analogues, the cell surface was modified to contain sialic acid with one of the following C-9 substituents: an azido, an amino, an acetamido, or a hexanoylamido group. Among these, only 9-acetamido-N-acetylneuraminic acid (9-acetamido-Neu5Ac) was able to function as a receptor determinant for influenza C virus as indicated by the ability of the virus to agglutinate the modified red blood cells. In contrast to the natural receptors, 9-acetamido-Neu5Ac-containing receptors were found to be resistant against the action of sialate 9-O-acetylesterase, the viral receptor-destroying enzyme. No difference in the hemolytic activity of influenza C virus was detected when analyzed with erythrocytes containing either Neu5,9Ac2 or 9-acetamido-Neu5Ac on their surface. This finding indicates that cleavage of the receptor is not required for the viral fusion activity. The sialic acid analogues should be useful for analyzing not only the importance of the receptor-destroying enzyme of influenza C virus, but also other biological processes involving sialic acid.
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- 1992
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10. A single point mutation of the influenza C virus glycoprotein (HEF) changes the viral receptor-binding activity
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Sigrun Szepanski, Hans-Dieter Klenk, Hans-Jürgen Gross, Reinhard Brossmer, and G. Herrler
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Influenzavirus C ,Molecular Sequence Data ,Mutant ,Orthomyxoviridae ,Hemagglutinins, Viral ,Hemagglutinin (influenza) ,Hemagglutinin Glycoproteins, Influenza Virus ,Biology ,Article ,Virus ,Cell Line ,chemistry.chemical_compound ,Dogs ,Viral Envelope Proteins ,Virology ,Animals ,Amino Acid Sequence ,Peptide sequence ,biology.organism_classification ,Sialic acid ,Kinetics ,chemistry ,Mutation ,biology.protein ,Receptors, Virus ,Influenza C Virus ,Neuraminidase - Abstract
From strain JHB/1/66 of influenza C virus a mutant was derived with a change in the cell tropism. The mutant was able to grow in a subline of Madin-Darby canine kidney cells (MDCK II) which is resistant to infection by the parent virus due to a lack of receptors. Inactivation of cellular receptors by either neuraminidase or acetylesterase and generation of receptors by resialylation of cells with N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2) indicated that 9-O-acetylated sialic acid is a receptor determinant for both parent and mutant virus. However, the mutant required less Neu5,9Ac2 on the cell surface for virus attachment than the parent virus. The increased binding efficiency enabled the mutant to infect cells with a low content of 9-O-acetylated sialic acid which were resistant to the parent virus. By comparing the nucleotide sequences of the glycoprotein (HEF) genes of the parent and the mutant virus only a single point mutation could be identified on the mutant gene. This mutation at nucleotide position 872 causes an amino acid exchange from threonine to isoleucine at position 284 on the amino acid sequence. Sequence similarity with a stretch of amino acids involved in the receptor-binding pocket of the influenza A hemagglutinin suggests that the mutation site on the influenza C glycoprotein (HEF) is part of the receptor-binding site.
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- 1992
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11. The S protein of bovine coronavirus is a hemagglutinin recognizing 9-O-acetylated sialic acid as a receptor determinant
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R Brossmer, B Schultze, G. Herrler, and H.J. Gross
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Aging ,Erythrocytes ,Coronaviridae ,Immunology ,Hemagglutinins, Viral ,Hemagglutinin (influenza) ,medicine.disease_cause ,Microbiology ,Cell Line ,chemistry.chemical_compound ,Viral Envelope Proteins ,Cell surface receptor ,Virology ,medicine ,Animals ,Humans ,Receptor ,Coronavirus ,Binding Sites ,biology ,Hemagglutinin esterase ,Viral membrane ,Bromelains ,N-Acetylneuraminic Acid ,Sialic acid ,Molecular Weight ,Biochemistry ,chemistry ,Insect Science ,Sialic Acids ,biology.protein ,Acetylesterase ,Cattle ,Electrophoresis, Polyacrylamide Gel ,Carboxylic Ester Hydrolases ,Chickens ,N-Acetylneuraminic acid ,Research Article - Abstract
The S protein of bovine coronavirus (BCV) has been isolated from the viral membrane and purified by gradient centrifugation. Purified S protein was identified as a viral hemagglutinin. Inactivation of the cellular receptors by sialate 9-O-acetylesterase and generation of receptors by sialylation of erythrocytes with N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2) indicate that S protein recognizes 9-O-acetylated sialic acid as a receptor determinant as has been shown previously for intact virions. The second glycoprotein of BCV, HE, which has been thought previously to be responsible for the hemagglutinating activity of BCV, is a less efficient hemagglutinin; it agglutinates mouse and rat erythrocytes, but in contrast to S protein, it is unable to agglutinate chicken erythrocytes, which contain a lower level of Neu5,9Ac2 on their surface. S protein is proposed to be responsible for the primary attachment of virus to cell surface. S protein is proposed to be responsible for the primary attachement of virus to cell surface receptors. The potential of S protein as a probe for the detection of Neu5,9Ac2-containing glycoconjugates is demonstrated.
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- 1991
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12. Isolated HE-protein from hemagglutinating encephalomyelitis virus and bovine coronavirus has receptor-destroying and receptor-binding activity
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B Schultze, Hans-Dieter Klenk, G. Herrler, and K. Wahn
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Virus Cultivation ,Coronaviridae ,Swine ,viruses ,Hemagglutinins, Viral ,Biology ,medicine.disease_cause ,Article ,Cell Line ,Viral Proteins ,Virology ,medicine ,Animals ,Hemagglutination, Viral ,Coronavirus ,Bovine coronavirus ,Hemagglutinin esterase ,Acetylesterase activity ,Acetylesterase ,Hemagglutination Tests ,Hemagglutinin ,Viral membrane ,Hemagglutination Inhibition Tests ,Molecular biology ,Agglutination (biology) ,Receptors, Virus ,Cattle ,Electrophoresis, Polyacrylamide Gel ,Viral Fusion Proteins - Abstract
Bovine coronavirus (BCV) and hemagglutinating encephalomyelitis virus (HEV) from swine were found to grow to high titers in MDCK I cells, a subline of Madin Darby canine kidney cells. Virus grown in these cells was used to isolate and purify the HE-protein. This protein has been shown recently to have acetylesterase activity and to function as the receptor-destroying enzyme of BCV. Here we show that HEV contains this enzyme, too. The glycoproteins were solubilized by treatment of virions with octylglucoside. Following centrifugation through a sucrose gradient the surface proteins S and HE (hemagglutinin-esterase) were obtained in purified form. After removal of the detergent by dialysis, HE formed rosettes as shown by electron microscopy. The purified HE protein retained acetylesterase activity and was able to function as a receptor-destroying enzyme rendering red blood cells resistant against agglutination by both coronaviruses. HE protein released from the viral membrane failed to agglutinate red blood cells. However, it was found to recognize glycoconjugates containing N-acetyl-9-O-acetylneuraminic acid as indicated by a binding assay with rat serum proteins blotted to nitrocellulose and by its ability to inhibit the hemagglutinating activity of BCV, HEV, and influenza C virus. The purified enzyme provides a useful tool for analyzing the cellular receptors for coronaviruses.
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- 1991
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13. The hemagglutinating glycoproteins of influenza B and C viruses are acylated with different fatty acids
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Michael Veit, Michael F. G. Schmidt, Rudolf Rott, Hans-Dieter Klenk, and G. Herrler
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Influenzavirus C ,Acylation ,viruses ,Orthomyxoviridae ,Palmitic Acid ,Hemagglutinins, Viral ,Hemagglutinin (influenza) ,Hemagglutinin Glycoproteins, Influenza Virus ,Hydroxylamine ,Palmitic Acids ,Hydroxylamines ,Myristic Acid ,Virus ,Cell Line ,Microbiology ,chemistry.chemical_compound ,Viral Envelope Proteins ,Virology ,Animals ,Amino Acids ,Mercaptoethanol ,chemistry.chemical_classification ,Glucosamine ,biology ,Influenzavirus B ,Fatty Acids ,virus diseases ,Fatty acid ,biology.organism_classification ,Influenza B virus ,Biochemistry ,chemistry ,biology.protein ,lipids (amino acids, peptides, and proteins) ,Stearic acid ,Influenza C Virus ,Myristic Acids ,Stearic Acids - Abstract
We present evidence that the hemagglutinin (HA) of influenza B virus and the glycoprotein of influenza C virus (HEF) are acylated. The fatty acid linkage is sensitive to treatment with hydroxylamine and mercaptoethanol, which points to a labile thioester-type linkage. The HA of influenza B virus contains mainly palmitic acid, whereas the HEF glycoprotein of influenza C virus is acylated with stearic acid which has not been observed before as the prevailing fatty acid in viral or cellular acyl proteins.
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- 1990
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14. Hemagglutinating encephalomyelitis virus attaches to N-acetyl-9-O-acetylneuraminic acid-containing receptors on erythrocytes: comparison with bovine coronavirus and influenza C virus
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Reinhard Brossmer, Hans-Jürgen Gross, Hans-Dieter Klenk, B Schultze, and G. Herrler
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Cancer Research ,Erythrocytes ,Influenzavirus C ,Hemagglutination ,Coronaviridae ,receptor ,viruses ,Biology ,medicine.disease_cause ,Article ,Virus ,Microbiology ,chemistry.chemical_compound ,Bovine coronavirus ,Virology ,medicine ,Animals ,Humans ,N-acetyl-9-O-acetylneuraminic acid ,Cells, Cultured ,Hemagglutination, Viral ,Coronavirus ,Hemagglutinating encephalomyelitis virus ,virus diseases ,Orthomyxoviridae ,Sialic acid ,Agglutination (biology) ,Infectious Diseases ,chemistry ,Sialic Acids ,Receptors, Virus ,Acetylesterase ,Influenza C Virus ,Carboxylic Ester Hydrolases - Abstract
The receptors for the hemagglutinating encephalomyelitis virus (HEV, a porcine coronavirus) on chicken erythrocytes were analyzed and compared to the receptors for bovine coronavirus (BCV) and influenza C virus. Evidence was obtained that HEV requires the presence of N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2) on the cell surface for agglutination of erythrocytes as has been previously shown for BCV and influenza C virus: (i) Incubation of red blood cells with sialate 9-O-acetylesterase, the receptor-destroying enzyme of influenza C virus, rendered the erythrocytes resistant against agglutination by each of the three viruses; (ii) Human erythrocytes which are resistant to agglutination by HEV acquire receptors for HEV after resialylation with Neu5,9Ac2. Sialylation of red blood cells with limiting amounts of sialic acid indicated that strain JHB/1/66 of influenza C virus requires less Neu5,9Ac2 for agglutination of erythrocytes than the two coronaviruses, both of which were found to be similar in their reactivity with Neu5,9Ac2-containing receptors.
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- 1990
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15. Transmissible gastroenteritis virus infection: a vanishing specter
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C, Schwegmann-Wessels and G, Herrler
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Epitopes ,Binding Sites ,Gastroenteritis, Transmissible, of Swine ,Swine ,Transmissible gastroenteritis virus ,Animals ,N-Acetylneuraminic Acid - Abstract
About twenty years ago, a new coronavirus, porcine respiratory coronavirus (PRCoV), was detected in swine herds. This virus is related to transmissible gastroenteritis virus (TGEV); however, it is not enteropathogenic but causes only minor respiratory symptoms. As PRCoV shares some epitopes for neutralizing antibodies with TGEV, it acts like a nature-made vaccine against TGEV resulting in a drastic reduction of TGE outbreaks in Europe. A major difference between the two porcine coronaviruses is a large deletion in the surface protein S gene of PRCoV. Because of this structural difference, TGEV but not PRCoV has a sialic acid binding activity that allows the attachment to mucins and mucin-type glycoproteins. The sialic acid binding activity may allow TGEV to overcome the mucus barrier in the gut and to get access to the intestinal epithelium for initiation of infection.
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- 2006
16. A sialic acid analogue acting as a receptor determinant for binding but not for infection by influenza C virus
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Rainer Isecke, Reinhard Brossmer, and G. Herrler
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Influenzavirus C ,Orthomyxoviridae ,Biophysics ,Biology ,Biochemistry ,Virus ,Cell Line ,chemistry.chemical_compound ,Dogs ,Structural Biology ,Influenza C virus ,Genetics ,Animals ,Molecular Biology ,chemistry.chemical_classification ,Molecular Structure ,Receptor determinant ,Cell Biology ,Acetylesterase ,biology.organism_classification ,Virology ,Sialic acid ,N-Acetyl-9-O-acetylneuraminic acid ,Enzyme ,chemistry ,Cell culture ,Sialic Acids ,Receptors, Virus ,Sialic acid analogue ,Influenza C Virus ,Chickens - Abstract
We describe a synthetic sialic acid analogue, 9-thioacetamido-N-acetylneuraminic acid (9-thioacetamido-Neu5Ac), which is recognized by the receptor-binding activity of influenza C virus, but is resistant to the receptor-destroying enzyme (acetylesterase) of this virus. Following transfer of the analogue to the surface of receptor-negative cells, influenza C virus is able to attach to these cells, but is unable to infect the cells. This result suggests that inactivation of virus receptors by the receptor-destroying enzyme is essential for initiation of infection. Because of their unique properties such analogues promise to be powerful chemotherapeutic agents.
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- 1993
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17. Proteolytic activation of respiratory syncytial virus fusion protein. Cleavage at two furin consensus sequences
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G, Zimmer, L, Budz, and G, Herrler
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Furin ,Sequence Homology, Amino Acid ,Hydrolysis ,Molecular Sequence Data ,Fluorescent Antibody Technique ,Cell Line ,Respiratory Syncytial Viruses ,Viral Proteins ,Chlorocebus aethiops ,Mutagenesis, Site-Directed ,Animals ,Amino Acid Sequence ,Subtilisins ,Vero Cells ,Viral Fusion Proteins - Abstract
The F (fusion) protein of the respiratory syncytial viruses is synthesized as an inactive precursor F(0) that is proteolytically processed at the multibasic sequence KKRKRR(136) into the subunits F(1) and F(2) by the cellular protease furin. This maturation process is essential for the F protein to gain fusion competence. We observed that proteolytic cleavage additionally occurs at another basic motif, RARR(109), that also meets the requirements for furin recognition. Cleavage at both sites leads to the removal from the polypeptide chain of a glycosylated peptide of 27 amino acids. When the sequence RARR(109) was changed to NANR(109) or to RANN(109) by site-directed mutagenesis, cleavage by furin was completely prevented. Although the mutants were still processed at position Arg(136), they did not show any syncytia formation. Proteolytic cleavage of the modified motifs was achieved by treatment of transfected cells with trypsin converting the F mutants into their fusogenic forms. Our findings indicate that both furin consensus sequences have to be cleaved in order to activate the fusion protein.
- Published
- 2001
18. Neuraminidase treatment of avian infectious bronchitis coronavirus reveals a hemagglutinating activity that is dependent on sialic acid-containing receptors on erythrocytes
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G. Herrler, B Schultze, and David Cavanagh
- Subjects
Erythrocytes ,animal structures ,Hemagglutination ,viruses ,Infectious bronchitis virus ,Hemagglutinins, Viral ,Neuraminidase ,In Vitro Techniques ,medicine.disease_cause ,Article ,Microbiology ,chemistry.chemical_compound ,Virology ,medicine ,Animals ,Coronavirus ,biology ,biology.organism_classification ,Avian infectious bronchitis ,Sialic acid ,Agglutination (biology) ,chemistry ,embryonic structures ,Sialic Acids ,biology.protein ,Receptors, Virus ,Avian infectious bronchitis virus ,Chickens - Abstract
The interaction of infectious bronchitis virus (IBV) with erythrocytes was analyzed. The binding activity of IBV was not sufficient to agglutinate chicken erythrocytes. However, it acquired hemagglutinating activity after treatment with neuraminidase to remove alpha 2,3-linked N-acetylneuraminic acid from the surface of the virion. Pretreatment of erythrocytes with neuraminidase rendered the cells resistant to agglutination by IBV. Susceptibility to agglutination was restored by resialylation of asialo-erythrocytes to contain alpha 2,3-linked sialic acid. These results indicate that IBV attaches to receptors on erythrocytes, the crucial determinant of which is sialic acid alpha 2,3-linked to galactose. In contrast to other enveloped viruses with such a binding specificity (influenza viruses and paramyxoviruses) IBV lacks a receptor-destroying enzyme.
- Published
- 1992
- Full Text
- View/download PDF
19. Importance of the carboxyl-terminal FTSL motif of membrane cofactor protein for basolateral sorting and endocytosis. Positive and negative modulation by signals inside and outside the cytoplasmic tail
- Author
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M, Teuchert, A, Maisner, and G, Herrler
- Subjects
Membrane Glycoproteins ,Recombinant Fusion Proteins ,Fluorescent Antibody Technique ,Gene Expression ,Hemagglutinins, Viral ,Transfection ,Endocytosis ,Peptide Fragments ,Cell Line ,Membrane Cofactor Protein ,Dogs ,Antigens, CD ,Influenza A virus ,Mutation ,Animals - Abstract
Membrane cofactor protein (MCP), a widely distributed complement regulatory protein, is expressed on the basolateral surface of polarized epithelial cells, and it is not endocytosed. The carboxyl-terminal tetrapeptide (FTSL) is required for polarized surface expression. The ability of this tetrapeptide to serve as an autonomous sorting signal has been analyzed by adding this sequence motif to the C terminus of an apical membrane protein, the influenza A virus hemagglutinin (HA). The recombinant protein HA-FTSL retained the apical localization of the parental HA protein. Substitution of the complete cytoplasmic tail of MCP for the cytoplasmic tail of HA resulted in the targeting of the chimeric protein (HA/MCP) to the basolateral surface suggesting that the carboxyl-terminal FTSL motif is a weak sorting signal that requires additional targeting information from the membrane-proximal part of the cytoplasmic tail of MCP for redirecting an apical protein to the basolateral membrane domain. In contrast to the native HA, the HA-FTSL protein was subject to endocytosis. The basolateral HA/MCP was also found to be internalized and thus differed from the basolateral MCP. This result suggests that the carboxyl-terminal FTSL motif serves as an internalization signal and that in native MCP sorting information outside the cytoplasmic tail counteracts this endocytosis signal. Substitution of a tyrosine for the phenylalanine dramatically increased the internalization with most of the HA-YTSL protein being present intracellularly. Our results are consistent with the view that the interplay of multiple sorting signals and the modification of a well known targeting signal (YTSL) by amino acid exchange (FTSL) determine the constitutive expression of MCP on the basolateral surface of polarized epithelial cells.
- Published
- 1999
20. Isolation of hemagglutination-defective mutants for the analysis of the sialic acid binding activity of transmissible gastroenteritis virus
- Author
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C, Krempl, M L, Ballesteros, L, Enjuanes, and G, Herrler
- Subjects
Swine ,Mutation ,Transmissible gastroenteritis virus ,Animals ,Defective Viruses ,Hemagglutination, Viral ,N-Acetylneuraminic Acid - Abstract
The surface protein S of transmissible gastroenteritis virus (TGEV) has a sialic acid binding activity that enables the virus to agglutinate erythrocytes. A protocol is described that has been successfully applied to the isolation of hemgglutination-defective mutants. The potential of these mutants for the characterization of the sialic acid-binding site and the function of the binding activity is discussed.
- Published
- 1998
21. Is the sialic acid binding activity of the S protein involved in the enteropathogenicity of transmissible gastroenteritis virus?
- Author
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C, Krempl, H, Laude, and G, Herrler
- Subjects
Swine Diseases ,Membrane Glycoproteins ,Viral Envelope Proteins ,Swine ,Spike Glycoprotein, Coronavirus ,Transmissible gastroenteritis virus ,Animals ,N-Acetylneuraminic Acid ,Gastroenteritis - Abstract
Transmissible gastroenteritis virus (TGEV) is able to recognize sialic acid on sialo-glycoconjugates. Analysis of mutants indicated that single point mutations in the S protein (around amino acids 145-155) of TGEV may result both in the loss of the sialic acid binding activity and in a drastic reduction of the enteropathogenicity. From this observation we conclude that the sialic acid binding activity is involved in the enteropathogenicity of TGEV. On the basis of our recent results we propose that binding of sialylated macromolecules to the virions surface may increase virus stability. This in turn would explain how TGEV as an enveloped virus can survive the gastrointestinal passage and cause intestinal infections.
- Published
- 1998
22. Polarized budding of measles virus is not determined by viral surface glycoproteins
- Author
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G. Herrler, Andrea Maisner, and Hans-Dieter Klenk
- Subjects
Protein Conformation ,viruses ,Immunology ,Microbiology ,Cell Line ,Measles virus ,Viral Proteins ,Dogs ,Viral envelope ,Virology ,Cell polarity ,Animals ,Epithelial polarity ,Glycoproteins ,chemistry.chemical_classification ,Budding ,biology ,Cell Polarity ,Biological Transport ,Epithelial Cells ,Apical membrane ,biology.organism_classification ,Virus Release ,Cell biology ,Virus-Cell Interactions ,chemistry ,Insect Science ,Glycoprotein - Abstract
For viruses that mature by a budding process, the envelope glycoproteins are considered the major determinants for the site of virus release from polarized epithelial cells. Viruses are usually released from that membrane domain where the viral surface glycoproteins are transported to. We here report that measles virus has developed a different maturation strategy. Measles virus was found to be released from the apical membrane domain of polarized epithelial cells, though the surface glycoproteins H and F were transported in a nonpolarized fashion and to the basolateral membrane domain, respectively.
- Published
- 1998
23. Membrane cofactor protein (CD46) is a basolateral protein that is not endocytosed. Importance of the tetrapeptide FTSL at the carboxyl terminus
- Author
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A, Maisner, G, Zimmer, M K, Liszewski, D M, Lublin, J P, Atkinson, and G, Herrler
- Subjects
Membrane Cofactor Protein ,Structure-Activity Relationship ,Dogs ,Membrane Glycoproteins ,Antigens, CD ,Molecular Sequence Data ,Animals ,Neuraminidase ,Biological Transport ,Amino Acid Sequence ,Oligopeptides ,Cells, Cultured ,Endocytosis - Abstract
Membrane cofactor protein (MCP) is a widely distributed complement regulatory protein that is expressed on the basolateral surface of polarized epithelial cells. The basolateral targeting of the BC1 isoform of MCP was analyzed by generating deletion mutants and point mutants within the cytoplasmic tail of 16 amino acids. A sequence of four amino acids, FTSL, was found to be indispensable for the basolateral transport of MCP. This tetrapeptide has two unique features compared with the targeting motifs of other basolateral proteins: (i) it contains a phenylalanine rather than a tyrosine at position 1; (ii) it is located at the very COOH-terminal end. Replacement of the phenylalanine or the leucine by an alanine resulted in a nonpolarized delivery to the cell surface. On the other hand, substitution of a tyrosine for the phenylalanine did not affect the basolateral transport of MCP. The latter mutant, however, was efficiently internalized, whereas the wild type protein was not subject to endocytosis. Our results indicate that the targeting signal YXX-large aliphatic that is involved in various sorting events has been modulated in MCP in such a way that it allows basolateral transport but not endocytosis.
- Published
- 1997
24. Point mutations in the S protein connect the sialic acid binding activity with the enteropathogenicity of transmissible gastroenteritis coronavirus
- Author
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B Schultze, H Laude, C. Krempl, and G. Herrler
- Subjects
Male ,Swine ,Immunology ,Transmissible gastroenteritis coronavirus ,Mutant ,Neuraminidase ,Sialic acid binding ,medicine.disease_cause ,Sialidase ,Microbiology ,Cell Line ,Viral Envelope Proteins ,Virology ,medicine ,Animals ,Point Mutation ,Coronavirus ,chemistry.chemical_classification ,Membrane Glycoproteins ,biology ,Point mutation ,Transmissible gastroenteritis virus ,biology.organism_classification ,Amino acid ,Hemagglutinins ,chemistry ,Insect Science ,Spike Glycoprotein, Coronavirus ,biology.protein ,Sialic Acids ,LLC-PK1 Cells ,Receptors, Virus ,Chickens ,Research Article - Abstract
Enteropathogenic transmissible gastroenteritis virus (TGEV), a porcine coronavirus, is able to agglutinate erythrocytes because of sialic acid binding activity. Competitive inhibitors that may mask the sialic acid binding activity can be inactivated by sialidase treatment of virions. Here, we show that TGEV virions with efficient hemagglutinating activity were also obtained when cells were treated with sialidase prior to infection. This method was used to analyze TGEV mutants for hemagglutinating activity. Recently, mutants with strongly reduced enteropathogenicity that have point mutations or a deletion of four amino acids within residues 145 to 155 of the S protein have been described. Here, we show that in addition to their reduced pathogenicity, these mutants also have lost hemagglutinating activity. These results connect sialic acid binding activity with the enteropathogenicity of TGEV.
- Published
- 1997
25. Two different cytoplasmic tails direct isoforms of the membrane cofactor protein (CD46) to the basolateral surface of Madin-Darby canine kidney cells
- Author
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John P. Atkinson, G. Herrler, Andrea Maisner, Reinhard Schwartz-Albiez, and M. Kathryn Liszewski
- Subjects
Signal peptide ,Gene isoform ,Cytoplasm ,Molecular Sequence Data ,Gene Expression ,Biology ,Protein Sorting Signals ,Kidney ,Transfection ,Biochemistry ,Cell Line ,Membrane Cofactor Protein ,Dogs ,Antigens, CD ,Chlorocebus aethiops ,Animals ,Humans ,Amino Acid Sequence ,Tyrosine ,Molecular Biology ,Vero Cells ,Membrane Glycoproteins ,Alternative splicing ,Cell Membrane ,Cell Polarity ,Cell Biology ,Cell biology ,Cell culture ,Biotinylation ,Mutation - Abstract
Membrane cofactor protein (MCP; CD46), a widely distributed regulatory protein of the complement system, was analyzed for expression in polarized epithelial cells. Both a human and a simian (Vero C1008) cell line were found to contain endogenous MCP mainly on the basolateral surface. Transfected Madin-Darby canine kidney cells stably expressing human MCP delivered this protein also predominantly to the basolateral surface. A deletion mutant lacking the cytoplasmic tail was transported in a nonpolarized fashion, indicating that the targeting signal for the basolateral transport is located in the cytoplasmic domain. A characteristic feature of MCP is the presence of various isoforms that contain either of two different cytoplasmic tails as a consequence of alternative splicing. Two isoforms differing only in the cytoplasmic tail (tail 1 or 2) were analyzed for polarized expression in Madin-Darby canine kidney cells. Surface biotinylation, as well as confocal immunofluorescence microscopy, indicated that both proteins were transported to the basolateral surface. Because no sequence similarity has been observed, the two tails contain different basolateral targeting signals. A deletion mutant lacking the only tyrosine residue in tail 1 retained the polarized expression indicating that, in contrast to most basolateral sorting signals, the transport signal of the tail 1 isoform is not dependent on tyrosine. The maintenance of a targeting motif in two distinct cytoplasmic tails suggests that the basolateral expression of MCP in polarized epithelial cells is of physiological importance.
- Published
- 1996
26. Structural and functional analysis of the S proteins of two human coronavirus OC43 strains adapted to growth in different cells
- Author
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F. Künkel and G. Herrler
- Subjects
viruses ,Molecular Sequence Data ,Infectious Disease ,Biology ,medicine.disease_cause ,Cell Line ,Coronavirus OC43, Human ,chemistry.chemical_compound ,Mice ,Dogs ,Viral Envelope Proteins ,Virology ,Chlorocebus aethiops ,medicine ,Animals ,Humans ,Human coronavirus OC43 ,Amino Acid Sequence ,Peptide sequence ,Vero Cells ,Coronavirus ,Bovine coronavirus ,chemistry.chemical_classification ,Coronavirus, Bovine ,Membrane Glycoproteins ,Base Sequence ,Sequence Homology, Amino Acid ,Brief Report ,Nucleic acid sequence ,Nucleotide Sequence ,General Medicine ,biology.organism_classification ,Adaptation, Physiological ,Amino acid ,Sialic acid ,chemistry ,DNA, Viral ,Spike Glycoprotein, Coronavirus ,Vero cell ,Sialic Acids ,RNA, Viral ,Receptors, Virus ,Cattle ,Nucleotide ,Functional Analysis - Abstract
Summary The receptor-binding activity of strain CU (grown in MDCK I cells) and of strain VA (adapted to Vero cells) of human coronavirus OC43 was analyzed and compared with the binding activity of bovine coronavirus (BCV) and of the OC43 strain provided by the American Type Culture Collection (AT). Results obtained with resialylated erythrocytes indicated that the ability of the viruses to recognize 9-O-acetylated sialic acid in an α2,6-linkage decreased in the following order: AT>CU>BCV>VA. Only minor differences were observed with respect to the α2,3-linkage. The amino acid sequence of the S protein of strain CU and VA was derived from the nucleotide sequence of the cloned gene. Strain VA differed from strain CU in 34 positions, 18 in the S1 and 16 in the S2 subunit.
- Published
- 1996
27. A synthetic sialic acid analog that is resistant to the receptor-destroying enzyme can be used by influenza C virus as a receptor determinant for infection of cells
- Author
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Hans-Jürgen Gross, Reinhard Brossmer, and G. Herrler
- Subjects
Influenzavirus C ,Cell ,Biophysics ,Biology ,Kidney ,Biochemistry ,Esterase ,Virus ,Cell Line ,chemistry.chemical_compound ,Structure-Activity Relationship ,Dogs ,medicine ,Cytidine Monophosphate ,Animals ,Receptor ,Molecular Biology ,chemistry.chemical_classification ,Molecular Structure ,Cell Membrane ,Esterases ,Cell Biology ,Acetylesterase ,Virology ,Sialic acid ,medicine.anatomical_structure ,Enzyme ,chemistry ,Sialic Acids ,Receptors, Virus ,Influenza C Virus - Abstract
A synthetic sialic acid analog, N-acetyl-9-acetamido-9-deoxy-neuraminic acid, can be used by influenza C virus as a receptor determinant for attachment to cells, In contrast to the natural determinant, N-acetyl-9-O-acetylneuraminic acid, the synthetic sialic acid is resistant to the action of the receptor-destroying acetylesterase of this virus. The sialic acid analog was enzymatically transferred to the surface of Madin-Darby canine kidney cells that are resistant to infection because of a lack of receptors. Influenza C virus was able to infect the modified cells though requiring a 10-fold larger amount of the sialic acid analogue on the cell surface compared to the natural receptor determinant. The quantitative difference is accounted for mainly by a less efficient binding of influenza C virus to the analog. Thus, in our system, inactivation of the receptor by the viral esterase is not required for the initiation of an influenza C virus infection.
- Published
- 1995
28. Membrane cofactor protein with different types of N-glycans can serve as measles virus receptor
- Author
-
G. Herrler and Andrea Maisner
- Subjects
Glycosylation ,1-Deoxynojirimycin ,Oligosaccharides ,Virus ,Measles virus ,Membrane Cofactor Protein ,chemistry.chemical_compound ,Antigens, CD ,Polysaccharides ,Virology ,Chlorocebus aethiops ,Animals ,Receptor ,Vero Cells ,Membrane Glycoproteins ,biology ,CD46 ,Tunicamycin ,biology.organism_classification ,Molecular biology ,carbohydrates (lipids) ,Molecular Weight ,Membrane glycoproteins ,Biochemistry ,chemistry ,Vero cell ,biology.protein ,Receptors, Virus ,Mannose - Abstract
Membrane cofactor protein (MCP) has been shown to act as a cellular receptor for measles virus. In previous binding studies we demonstrated a direct interaction between the measles virus H protein and MCP. The binding was shown to be independent of the O-glycans but dependent on the N-glycans of MCP. To elucidate the role of N-glycans for the receptor function of MCP, the effect of the glycosylation inhibitors tunicamycin (TM) and 1-deoxymannojirimycin (DMJ) was analyzed. TM which prevents N-glycosylation has been reported to inhibit the expression of functional measles virus receptors. Here we show that MCP lacking all N-glycans was detectable on the surface of Vero cells, although in a reduced amount. Therefore, the lack of receptor activity cannot be explained by intracellular degradation or defective transport. In the presence of DMJ, a mannosidase I inhibitor, MCP is synthesized with N-glycans of the high-mannose type in contrast to the complex oligosaccharides present on MCP of untreated cells. Both MCP with mannose-rich and MCP with complex N-glycans were recognized by measles virus H protein in an in vitro binding assay. They both could also serve as receptors for the infection of cultured Vero cells, arguing against a direct binding of virus to a carbohydrate moiety within the N-glycans of MCP. We propose that N-linked oligosaccharides are required to maintain a conformation-dependent receptor determinant of MCP.
- Published
- 1995
29. Analysis of cellular receptors for human coronavirus OC43
- Author
-
C, Krempl, B, Schultze, and G, Herrler
- Subjects
Coronavirus, Bovine ,Erythrocytes ,Hemagglutination ,Molecular Sequence Data ,Cell Line ,Coronavirus ,Coronavirus OC43, Human ,Carbohydrate Sequence ,Carbohydrate Conformation ,Sialic Acids ,Animals ,Humans ,Receptors, Virus ,Cattle - Abstract
Bovine coronavirus (BCV), human coronavirus OC43 (HCV-OC43) and hemagglutinating encephalomyelitis virus (HEV) are serologically related viruses that all have hemagglutinating activity. The receptor determinant for attachment to erythrocytes has been shown to be N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2). We compared the ability of the three coronaviruses to recognize 9-O-acetylated sialic acid and found that they all bind to Neu5,9Ac2 attached to galactose in either A2,3 or A2,6-linkage. There are, however, some differences in the minimum amount of sialic acid that is required on the cell surface for agglutination by these viruses. Evidence is presented that HCV-OC43 uses Neu5,9Ac2 as a receptor determinant not only for agglutination of erythrocytes but also for attachment to and infection of a cultured cell line, MDCK I cells.
- Published
- 1995
30. Analysis of the Sialic Acid-Binding Activity of Transmissible Gastroenteritis Virus
- Author
-
G. Herrler, Luis Enjuanes, and B Schultze
- Subjects
chemistry.chemical_compound ,Hemagglutination assay ,Hemagglutination ,chemistry ,biology ,Neuraminic acid ,biology.protein ,Sialic acid binding ,N-Acetylneuraminic acid ,Virology ,Neuraminidase ,Virus ,Sialic acid - Abstract
Porcine transmissible gastroenteritis virus (TGEV) has been shown to agglutinate erythrocytes using a2,3-linked sialic acid on the cell surface as binding site. The hemagglutinating activity requires the pretreament of virus with neuraminidase. We obtained evidence that TGEV recognizes not only N-acetylneuraminic acid but also N-glycoloylneuraminic acid, a sialic acid present on many porcine cells.
- Published
- 1995
- Full Text
- View/download PDF
31. Analysis of Cellular Receptors for Human Coronavirus OC43
- Author
-
C. Krempl, B Schultze, and G. Herrler
- Subjects
biology ,viruses ,Encephalomyelitis ,Cell ,virus diseases ,medicine.disease ,biology.organism_classification ,Virology ,Virus ,Sialic acid ,Agglutination (biology) ,chemistry.chemical_compound ,medicine.anatomical_structure ,chemistry ,medicine ,Human coronavirus OC43 ,Receptor ,Bovine coronavirus - Abstract
Bovine coronavirus (BCV), human coronavirus OC43 (HCV-OC43) and hemagglutinating encephalomyelitis virus (HEV) are serologically related viruses that all have hemagglutinating activity. The receptor determinant for attachment to erythrocytes has been shown to be N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2). We compared the ability of the three coronaviruses to recognize 9-O-acetylated sialic acid and found that they all bind to Neu5,9Ac2 attached to galactose in either A2,3 or A2,6-linkage. There are, however, some differences in the minimum amount of sialic acid that is required on the cell surface for agglutination by these viruses. Evidence is presented that HCV-OC43 uses Neu5,9Ac2 as a receptor determinant not only for agglutination of erythrocytes but also for attachment to and infection of a cultured cell line, MDCK I cells.
- Published
- 1995
- Full Text
- View/download PDF
32. Polarized entry of bovine coronavirus in epithelial cells
- Author
-
B, Schultze and G, Herrler
- Subjects
Coronavirus, Bovine ,Dogs ,Influenzavirus C ,Species Specificity ,Hemagglutination ,Cell Membrane ,Animals ,Cattle ,Chick Embryo ,Epithelium ,Cell Line - Abstract
Epithelial cells are highly polarized cells divided into an apical and a basolateral plasma membrane. The two domains are composed of a distinct set of proteins and lipids. Concerning virus infection of epithelial cells, the polarity of host cell receptor distribution defines the domain from which infection may be mediated. We were interested to analyze the infection of polarized cells by bovine coronavirus (BCV). The entry of BCV into MDCK I cells was investigated by growing the cells on a permeable support. Cell were infected with BCV from either the apical or basolateral domain. The efficiency of infection was determined by measuring the hemaglutinating activity of the virus released into the apical compartment. Virus replication was only detectable after inoculation from the apical surface. Therefore, infection of MDCK I cells with BCV is restricted to the apical side.
- Published
- 1995
33. Sialic Acid as Receptor Determinant of Ortho- and Paramyxoviruses
- Author
-
Hans-Dieter Klenk, G. Herrler, and Jürgen Hausmann
- Subjects
chemistry.chemical_classification ,biology ,viruses ,Hemagglutinin (influenza) ,Mumps virus ,medicine.disease_cause ,biology.organism_classification ,Sialidase ,Virology ,Sendai virus ,Virus ,Sialic acid ,chemistry.chemical_compound ,Biochemistry ,chemistry ,medicine ,biology.protein ,Glycoprotein ,Influenza C Virus - Abstract
The designation myxoviruses has been chosen historically for a group of viruses comprising influenza viruses, Newcastle disease virus, and mumps virus, because they were able to interact with mucins (see Chapter 5). A characteristic feature of these viruses was the presence of two activities that appeared to counteract each other. On the one hand, the viruses bind to receptors present on erythrocytes, resulting in a hemagglutination reaction. On the other hand, they contain a receptor-destroying enzyme rendering erythrocytes resistant to the viral agglutinating activity. The receptor determinant recognized by this group of viruses turned out to be sialic acid, and the receptor-destroying enzyme has been characterized as a sialidase and a sialate O-acetylesterase. Despite the similarities, members of the myxovirus group differ in several fundamental aspects, e.g., the presence of a segmented or a nonsegmented genome. Therefore, they have been grouped into two taxonomic families. Influenza A, B, and C viruses belong to the family Orthomyxoviridae. Viruses such as mumps virus, Newcastle disease virus, Sendai virus, and other parainfluenza viruses are members of the family Paramyxoviridae. In addition to the receptor-binding and the receptor-destroying activity, these viruses have a fusion activity. They differ, however, in the distribution of the three activities on the viral surface glycoproteins. With influenza A and B viruses, receptor-binding and fusion activity are functions of the hemagglutinin (HA). A second glycoprotein (NA) is responsible for the sialidase activity. In the case of paramyxoviruses, the receptor-binding and the sialidase activity are combined on one type of glycoprotein designated HN, whereas the fusion activity is localized on a separate glycoprotein (F). Influenza C viruses have only a single glycoprotein that is responsible for all three activities. They also differ from the other viruses in that they recognize N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2) rather than N-acetylneuraminic acid (Neu5Ac) as receptor determinant. Furthermore, the receptor-destroying enzyme of influenza C viruses is a sialate 9-O-acetylesterase. In this chapter, the interaction of viral proteins with sialic acid and the biological significance of the receptor-binding and the receptor-destroying activity are discussed.
- Published
- 1995
- Full Text
- View/download PDF
34. Analysis of the sialic acid-binding activity of the transmissible gastroenteritis virus
- Author
-
B, Schultze, L, Enjuanes, and G, Herrler
- Subjects
Binding Sites ,Erythrocytes ,Molecular Structure ,Swine ,Hemagglutination ,Transmissible gastroenteritis virus ,Neuraminidase ,N-Acetylneuraminic Acid ,Cell Line ,Sialic Acids ,Animals ,Cattle ,Neuraminic Acids ,Chickens - Abstract
Porcine transmissible gastroenteritis virus (TGEV) has been shown to agglutinate erythrocytes using alpha 2,3-linked sialic acid on the cell surface as binding site. The hemagglutinating activity requires the pretreatment of virus with neuraminidase. We obtained evidence that TGEV recognizes not only N-acetylneuraminic acid but also N-glycoloylneuraminic acid, a sialic acid present on many porcine cells.
- Published
- 1995
35. Polarized Entry of Bovine Coronavirus in Epithelial Cells
- Author
-
B Schultze and G. Herrler
- Subjects
medicine.anatomical_structure ,Polarity (international relations) ,Viral replication ,Chemistry ,Cell ,medicine ,Apical compartment ,Basolateral plasma membrane ,Receptor ,Virus ,Cell biology ,Bovine coronavirus - Abstract
Epithelial cells are highly polarized cells divided into an apical and a basolateral plasma membrane. The two domains are composed of a distinct set of proteins and lipids. Concerning virus infection of epithelial cells, the polarity of host cell receptor distribution defines the domain from which infection may be mediated. We were interested to analyze the infection of polarized cells by bovine coronavirus (BCV). The entry of BCV into MDCK I cells was investigated by growing the cells on a permeable support. Cell were infected with BCV from either the apical or basolateral domain. The efficiency of infection was determined my measuring the hemaglutinating activity of the virus released into the apical compartment. Virus replication was only detectable after inoculation from the apical surface. Therefore, infection of MDCK I cells with BCV is restricted to the apical side.
- Published
- 1995
- Full Text
- View/download PDF
36. Binding of measles virus to membrane cofactor protein (CD46): importance of disulfide bonds and N-glycans for the receptor function
- Author
-
M.K. Liszewski, G. Herrler, John P. Atkinson, Jurgen Schneider-Schaulies, and Andrea Maisner
- Subjects
Moesin ,viruses ,Immunology ,Blotting, Western ,Biotin ,Oligosaccharides ,Kidney ,Microbiology ,Virus ,Cell Line ,Measles virus ,Cell membrane ,Membrane Cofactor Protein ,chemistry.chemical_compound ,Antigens, CD ,Polysaccharides ,Virology ,Chlorocebus aethiops ,medicine ,Tumor Cells, Cultured ,Animals ,Humans ,ddc:610 ,Disulfides ,Vero Cells ,Membrane Glycoproteins ,biology ,CD46 ,Rectal Neoplasms ,Cell Membrane ,biology.organism_classification ,Molecular biology ,Sialic acid ,Membrane glycoproteins ,medicine.anatomical_structure ,chemistry ,Insect Science ,Vero cell ,biology.protein ,Sialic Acids ,HeLa Cells ,Research Article - Abstract
Two cellular proteins, membrane cofactor protein (MCP) and moesin, were reported recently to be functionally associated with the initiation of a measles virus infection. We have analyzed the interaction of measles virus with cell surface proteins, using an overlay binding assay with cellular proteins immobilized on nitrocellulose. Among surface-biotinylated proteins from a human rectal tumor cell line (HRT), measles virus was able to bind only to a 67-kDa protein that was identified as MCP. The virus recognized different isoforms of MCP expressed from human (HRT and HeLa) and simian (Vero) cell lines. The binding of measles virus to MCP was abolished after cleavage of the disulfide bonds by reducing agents as well as after enzymatic release of N-linked oligosaccharides. By contrast, removal of sialic acid or O-linked oligosaccharides did not affect the recognition of MCP measles virus. These data indicate that the receptor determinant of MCP is dependent on a conformation of the protein that is maintained by disulfide bonds and N-glycans present in the complement binding domains. Our results are consistent with a role of MCP as primary attachment site for measles virus in the initial stage of an infection. The functional relationship between MCP and moesin in a measles virus infection is discussed.
- Published
- 1994
37. N-Acetylneuraminic Acid Plays a Critical Role for the Haemagglutinating Activity of Avian Infectious Bronchitis Virus and Porcine Transmissible Gastroenteritis Virus
- Author
-
B Schultze, G. Herrler, Dave Cavanagh, and Luis Enjuanes
- Subjects
animal structures ,biology ,Hemagglutination ,viruses ,Infectious bronchitis virus ,biology.organism_classification ,medicine.disease_cause ,Virology ,Virus ,Sialic acid ,chemistry.chemical_compound ,chemistry ,Veterinary virology ,medicine ,biology.protein ,Avian infectious bronchitis virus ,Neuraminidase ,Coronavirus - Abstract
Porcine transmissible gastroenteritis virus (TGEV) was found to resemble avian infectious bronchitis virus (IBV) in its interaction with erythrocytes. Inactivation of the receptors on erythrocytes by neuraminidase treatment and restoration of receptors by reattaching N-acetylneuraminic acid (Neu5Ac) to cell surface components indicated that alpha 2,3-linked Neu5Ac serves as a receptor determinant for TGEV as has been reported recently for IBV. Similar to IBV, the haemagglutinating activity of TGEV is evident only after pretreatment of virus with neuraminidase indicating that inhibitors on the virion surface have to be inactivated in order to induce the HA-activity of these viruses. A model is presented to explain why the HA-activity of untreated virus is masked and how neuraminidase treatment results in the unmasking of this activity.
- Published
- 1994
- Full Text
- View/download PDF
38. Recognition of N-acetyl-9-O-Acetylneuraminic Acid by Bovine Coronavirus and Hemagglutinating Encephalomyelitis Virus
- Author
-
G. Herrler and B Schultze
- Subjects
biology ,Chemistry ,viruses ,Encephalomyelitis ,Ligand binding assay ,Hemagglutinin (influenza) ,Acetylesterase ,medicine.disease ,medicine.disease_cause ,Virology ,Virus ,Sialic acid ,chemistry.chemical_compound ,medicine ,biology.protein ,Bovine coronavirus ,Coronavirus - Abstract
The S protein of hemagglutinating encephalomyelitis virus is shown to be a hemagglutinin requiring N-acetyl-9-O-acetylneuraminic acid as a receptor determinant on the surface of erythrocytes. The ability of bovine coronavirus to recognize 9-O-acetylated sialic acid was used to establish a binding assay for the detection of glycoproteins containing this type of sugar. The assay is very fast, because it uses the acetylesterase of the viral HE protein to localize bound virus.
- Published
- 1994
- Full Text
- View/download PDF
39. Recognition of cellular receptors by bovine coronavirus
- Author
-
G. Herrler and B. Schultze
- Subjects
chemistry.chemical_classification ,Plasma protein binding ,Biology ,medicine.disease_cause ,Virology ,Sialic acid ,chemistry.chemical_compound ,Biochemistry ,chemistry ,Cell surface receptor ,medicine ,biology.protein ,Receptor ,Glycoprotein ,Neuraminidase ,Coronavirus ,Bovine coronavirus - Abstract
Bovine coronavirus (BCV) initiates infection by attachment to cell surface receptors the crucial component of which is N-acetyl-9-O- acetylneuraminic acid. Inactivation of receptors by neuraminidase treatment and restoration of receptors by enzymatic resialylation of asialo-cells is described as a method to determine (i) the type of sialic acid that is recognized; (ii) the linkage specificity of the viral binding activity; (iii) the minimal amount of sialic acid required for virus attachment. Evidence is presented that both glycoproteins and glycolipids can serve as receptors for BCV provided they contain 9-O-acetylated sialic acid. A model is introduced proposing that after initial binding to sialic acid-containing receptors, the S-protein of BCV interacts with a specific protein receptor. This interaction may result in a conformational change that exposes a fusogenic domain and thus induces the fusion between the viral and the cellular membrane.
- Published
- 1994
- Full Text
- View/download PDF
40. Recognition of cellular receptors by bovine coronavirus
- Author
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B, Schultze and G, Herrler
- Subjects
Coronavirus, Bovine ,Influenzavirus C ,Membrane Glycoproteins ,Carbohydrate Sequence ,Viral Envelope Proteins ,Molecular Sequence Data ,Spike Glycoprotein, Coronavirus ,Sialic Acids ,Receptors, Virus ,Glycolipids ,Glycoproteins ,Protein Binding ,Receptors, Coronavirus - Abstract
Bovine coronavirus (BCV) initiates infection by attachment to cell surface receptors the crucial component of which is N-acetyl-9-O-acetylneuraminic acid. Inactivation of receptors by neuraminidase treatment and restoration of receptors by enzymatic resialylation of asialo-cells is described as a method to determine (i) the type of sialic acid that is recognized; (ii) the linkage specificity of the viral binding activity; (iii) the minimal amount of sialic acid required for virus attachment. Evidence is presented that both glycoproteins and glycolipids can serve as receptors for BCV provided they contain 9-O-acetylated sialic acid. A model is introduced proposing that after initial binding to sialic acid-containing receptors, the S-protein of BCV interacts with a specific protein receptor. This interaction may result in a conformational change that exposes a fusogenic domain and thus induces the fusion between the viral and the cellular membrane.
- Published
- 1994
41. Surface glycoprotein of influenza C virus: inactivation and restoration of the acetylesterase activity on nitrocellulose
- Author
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Birgit Döll, Gert Zimmer, Stephan Pleschka, and G. Herrler
- Subjects
Cancer Research ,Protein Denaturation ,Influenzavirus C ,Orthomyxoviridae ,Viral Envelope Proteins ,Virology ,Bovine serum albumin ,chemistry.chemical_classification ,Gel electrophoresis ,biology ,Collodion ,Acetylesterase activity ,Serum Albumin, Bovine ,Acetylesterase ,Hydrogen-Ion Concentration ,biology.organism_classification ,Molecular biology ,Enzyme assay ,Enzyme Activation ,Infectious Diseases ,Biochemistry ,chemistry ,biology.protein ,Electrophoresis, Polyacrylamide Gel ,Influenza C Virus ,Glycoprotein - Abstract
The influenza C glycoprotein HEF was analyzed for acetylesterase activity after SDS-polyacrylamide gel electrophoresis and transfer to nitrocellulose membranes. Using a histological esterase assay, the glycoprotein was detected as a colored band indicating that it is enzymatically active. The enzyme activity was not affected by low pH, but was abolished after denaturation by SDS as well as after breaking the disulfide bonds by reducing agents. Glycoprotein inactivated by SDS regained its enzyme activity if the ionic detergent was displaced by either bovine serum albumin or a nonionic detergent. The stability of the enzyme combined with the color assay provides a convenient tool to study the acetylesterase activity of the influenza C virus glycoprotein.
- Published
- 1993
42. Structural and functional analysis of the surface protein of human coronavirus OC43
- Author
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G. Herrler and Frank Künkel
- Subjects
Viral protein ,Coronaviridae ,viruses ,Molecular Sequence Data ,Hemagglutinin (influenza) ,Hemagglutinins, Viral ,medicine.disease_cause ,Article ,chemistry.chemical_compound ,Viral Envelope Proteins ,Virology ,Agglutination Tests ,Viral structural protein ,medicine ,Tumor Cells, Cultured ,Animals ,Humans ,Human coronavirus OC43 ,Amino Acid Sequence ,Cloning, Molecular ,Bovine coronavirus ,Coronavirus ,Membrane Glycoproteins ,biology ,Base Sequence ,virus diseases ,biology.organism_classification ,N-Acetylneuraminic Acid ,Sialic acid ,chemistry ,Biochemistry ,DNA, Viral ,Spike Glycoprotein, Coronavirus ,biology.protein ,Sialic Acids ,N-Acetylneuraminic acid ,Chickens ,Protein Binding - Abstract
The two surface glycoproteins S and HE of human coronavirus OC43 (HCV-OC43) were isolated from the viral membrane and purified. Only the S protein was able to agglutinate chicken erythrocytes, indicating that this viral protein is the major hemagglutinin of HCV-OC43. The receptor determinant recognized by this virus on the surface of erythrocytes is N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2) which is also used by bovine coronavirus for attachment to cells. By analyzing erythrocytes containing different amounts of Neu5,9Ac2 in either of two linkage types, it was found that there are subtle differences in the affinity of both viruses for 9-O-acetylated sialic acid. Bovine coronavirus was more efficient in recognizing low amounts of Neu5,9Ac2 alpha 2,3 linked to galactose, whereas HCV-OC43 was superior with respect to the alpha 2,6 linkage. The gene coding for the S protein of HCV-OC43 was cloned and sequenced. A large open reading frame predicts a polypeptide of 150 kDa in the unglycosylated form. A protein of about 190 kDa is expected if the 20 potential glycosylation sites are used for attachment of N-linked oligosaccharide side chains. These predictions were confirmed by in vitro transcription and translation of the gene in the presence or absence of canine pancreatic microsomal membranes. A high degree of sequence homology was found between the S proteins of HCV-OC43 and bovine coronavirus. Structural and functional analyses of more strains should help to identify the location of the sialic acid-binding site.
- Published
- 1993
43. Viral Lectins for the Detection of 9-O-Acetylated Sialic Acid on Glycoproteins and Glycolipids
- Author
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G. Herrler, B. Schultze, and G. Zimmer
- Subjects
chemistry.chemical_classification ,chemistry.chemical_compound ,Biochemistry ,Chemistry ,Glycoconjugate ,viruses ,Asialoglycoprotein receptor ,Acetylesterase activity ,Acetylesterase ,Sialidase ,Influenza C Virus ,Bovine coronavirus ,Sialic acid - Abstract
A number of viruses are able to recognize specific carbohydrate structures and to use these structures for the attachment to the cell surface. Influenza C virus and bovine coronavirus specifically attach to receptors containing N-acetyl-9-O-acetylneuraminic acid. Therefore, they can be used as lectins for the detection of glycoconjugates containing this type of sialic acid. These viruses also contain an acetylesterase on their surface which can be exploited for the detection of virions bound to immobilized glycoconjugates (Zimmer et al. 1992). As shown in Fig. 1, in the case of influenza C virus the acetylesterase activity is a function of the surface glycoprotein HEF that also mediates the binding to N-acetyl-9-O-acetylneuraminic acid. In the case of bovine coronavirus the acetylesterase is a function of the HE protein. Though this protein also recognizes 9-O-acetylated sialic acid, the binding of virus is primarily due to a another surface glycoprotein designated S (Schultze et al. 1991). The esterases of both viruses are able to cleave the synthetic substrate α-naphthyl acetate giving rise to naphthol. The latter compound reacts with a diazonium ion such as Fast Red resulting in a coloured insoluble complex, which reveals the presence of bound virus.
- Published
- 1993
- Full Text
- View/download PDF
44. N-acetylneuraminic acid plays a critical role for the haemagglutinating activity of avian infectious bronchitis virus and porcine transmissible gastroenteritis virus
- Author
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B, Schultze, L, Enjuanes, D, Cavanagh, and G, Herrler
- Subjects
Membrane Glycoproteins ,Erythrocyte Membrane ,Infectious bronchitis virus ,Molecular Sequence Data ,Transmissible gastroenteritis virus ,Neuraminidase ,N-Acetylneuraminic Acid ,Bacterial Proteins ,Carbohydrate Sequence ,Viral Envelope Proteins ,Spike Glycoprotein, Coronavirus ,Sialic Acids ,Receptors, Virus ,Hemagglutination, Viral ,Receptors, Coronavirus - Abstract
Porcine transmissible gastroenteritis virus (TGEV) was found to resemble avian infectious bronchitis virus (IBV) in its interaction with erythrocytes. Inactivation of the receptors on erythrocytes by neuraminidase treatment and restoration of receptors by reattaching N-acetylneuraminic acid (Neu5Ac) to cell surface components indicated that alpha 2,3-linked Neu5Ac serves as a receptor determinant for TGEV as has been reported recently for IBV. Similar to IBV, the haemagglutinating activity of TGEV is evident only after pretreatment of virus with neuraminidase indicating that inhibitors on the virion surface have to be inactivated in order to induce the HA-activity of these viruses. A model is presented to explain why the HA-activity of untreated virus is masked and how neuraminidase treatment results in the unmasking of this activity.
- Published
- 1993
45. Recognition of N-acetyl-9-O-acetylneuraminic acid by bovine coronavirus and hemagglutinating encephalomyelitis virus
- Author
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B, Schultze and G, Herrler
- Subjects
Coronavirus, Bovine ,Membrane Glycoproteins ,Hemagglutinins, Viral ,Blood Proteins ,Hemagglutination Tests ,Cell Line ,Rats ,Coronavirus ,Viral Proteins ,Dogs ,Viral Envelope Proteins ,Spike Glycoprotein, Coronavirus ,Sialic Acids ,Animals ,Receptors, Virus ,Biological Assay ,Cattle ,Chickens ,Viral Fusion Proteins ,Glycoproteins ,Protein Binding ,Receptors, Coronavirus - Abstract
The S protein of hemagglutinating encephalomyelitis virus is shown to be a hemagglutinin requiring N-acetyl-9-O-acetylneuraminic acid as a receptor determinant on the surface of erythrocytes. The ability of bovine coronavirus to recognize 9-O-acetylated sialic acid was used to establish a binding assay for the detection of glycoproteins containing this type of sugar. The assay is very fast, because it uses the acetylesterase of the viral HE protein to localize bound virus.
- Published
- 1993
46. Monoclonal antibodies differentiate between the haemagglutinating and the receptor-destroying activities of bovine coronavirus
- Author
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Rudolf Rott, J. Storz, D. R. Snodgrass, M. A. Clark, G. Herrler, X. M. Zhang, and K. A. Hussain
- Subjects
Hemagglutination Inhibition Tests ,Erythrocytes ,Hemagglutination ,medicine.drug_class ,Coronaviridae ,Hemagglutinins, Viral ,medicine.disease_cause ,Monoclonal antibody ,Microbiology ,Viral Proteins ,Viral Envelope Proteins ,Virology ,medicine ,Animals ,Coronavirus ,Bovine coronavirus ,chemistry.chemical_classification ,biology ,Antibodies, Monoclonal ,Hemagglutinin ,Hemagglutinins ,chemistry ,biology.protein ,Sialic Acids ,Receptors, Virus ,Antibody ,Glycoprotein ,Chickens ,Viral Fusion Proteins - Abstract
A relatively simple and sensitive method is described which enables the effect of monoclonal antibodies (MAbs) on the receptor-destroying enzyme (RDE) and the haemagglutination (HA) activity of bovine coronavirus (BCV) to be analysed in one assay. A lysate of HRT-18 cells infected with the L9 strain of BCV was found to have a higher RDE:HA ratio than purified virus. At 4 degrees C the lysate induced an HA pattern which completely disappeared upon raising of the temperature to 37 degrees C. This L9-infected cell lysate was used to determine the HA inhibition (HAI) titres of MAbs directed against the surface glycoproteins S and HE of BCV. Thereafter, the test plates were incubated at 37 degrees C to enable the ability of the MAbs to prevent elution of virus from BCV-erythrocyte complexes to be assessed. No inhibition of RDE was detectable with MAbs against glycoprotein S, which had HAI titres ranging from 1:16 to 1:128. On the other hand, MAbs directed against glycoprotein HE had similar HAI titres, but they inhibited elution of 8 HA units of BCV at titres of up to 1:65,000.
- Published
- 1991
47. 9-O-acetylated sialic acid, a receptor determinant for influenza C virus and coronaviruses
- Author
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G, Herrler, S, Szepanski, and B, Schultze
- Subjects
Influenzavirus C ,Carbohydrate Sequence ,Coronaviridae ,Molecular Sequence Data ,Sialic Acids ,Animals ,Receptors, Virus ,Cell Line - Abstract
Influenza C virus and a group of coronaviruses, a typical representative of which is bovine coronavirus, use the same strategy for binding to cells. Surface components containing 9-O-acetylated sialic acid are recognized as cellular receptors by these viruses. In addition to the receptor determinant both virus groups have a receptor-destroying enzyme in common, which has been identified as a sialate 9-O-acetylesterase. Differences are, however, found in the distribution of these activities on the viral surface proteins. The influenza C glycoprotein HEF is a multifunctional protein, which is responsible for receptor-binding, receptor-inactivation and fusion. In the case of coronaviruses these activities are functions of two different glycoproteins, S and HE.
- Published
- 1991
48. Use of a sialic acid analogue to analyze the importance of the receptor-destroying enzyme for the interaction of influenza C virus with cells
- Author
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G, Herrler, H J, Gross, G, Milks, J C, Paulson, H D, Klenk, and R, Brossmer
- Subjects
Erythrocyte Aggregation ,Erythrocytes ,Influenzavirus C ,Orthomyxoviridae Infections ,Sialic Acids ,Animals ,Receptors, Virus ,Acetylesterase ,Chickens ,beta-D-Galactoside alpha 2-6-Sialyltransferase ,Sialyltransferases ,Glycoproteins - Abstract
Influenza C virus uses 9-O-acetyl-N-acetylaneuraminic acid (9-O-acetyl-Neu5Ac) as a receptor determinant for attachment to cells. The virus contains an acetylesterase which releases acetyl residues from position C-9 of sialic acid thereby inactivating the receptors. A synthetic sialic acid analogue, 9-N-acetyl-Neu5Ac, was attached to cell surface glycoconjugates by purified sialyltransferase and analyzed for its ability to substitute the 9-O-acetylated sialic acid. Erythrocytes which have been modified to contain either 9-O-acetyl-Neu5Ac or 9-N-acetyl-Neu5Ac were agglutinated by influenza C virus to the same titer. However, in contrast to the 9-O-acetyl group the 9-N-acetyl residue is resistant to cleavage by the viral acetylesterase. This characteristic property (recognition as a receptor determinant by influenza C virus, but resistance against the action of the receptor-destroying enzyme) makes this synthetic analogue a valuable tool to analyze the role of the receptor-destroying enzyme for an influenza C virus infection.
- Published
- 1990
49. Isolation and Characterization of the Acetylesterase of Hemagglutinating Encephalomyelitis Virus (HEV)
- Author
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G Hess, B Schultze, Hans-Dieter Klenk, Rudolf Rott, and G. Herrler
- Subjects
biology ,viruses ,Acetylesterase ,biology.organism_classification ,Virology ,Virus ,Sialic acid ,chemistry.chemical_compound ,Mouse hepatitis virus ,chemistry ,Neuraminic acid ,biology.protein ,Influenza C Virus ,Neuraminidase ,Bovine coronavirus - Abstract
Receptor-destroying enzymes have long been thought to be present only on influenza viruses and paramyxoviruses but not on other animal viruses. Paramyxoviruses as well as influenza A and B viruses are able to inactivate their own receptors by virtue of a neuraminidase which cleaves terminal sialic acid from glycoproteins or gangliosides (Drzeniek, 1972). The corresponding enzyme of influenza C virus is a sialate 9-0-acetylesterase which releases acetyl residues from position C-9 of N-acetyl-9-O-acetyl-neuraminic acid (Neu5,9Ac2) (Herrler et al., 1985). Recently, sequencing of the genome of mouse hepatitis virus revealed an open reading frame which surprisingly showed some similarity to the glycoprotein HEF of influenza C virus (Luytjes et al., 1988). This finding prompted a search which resulted in the discovery that bovine Coronavirus (BCV) contains a sialate O-acetylesterase similar to the receptor-destroying enzyme of influenza C virus (Vlasak et al., 1988a). This enzyme is inhibited by diisopropylfluorophos-phate (DFP), which binds covalently to serine in the active-site of serine proteases and esterases. By using a radioactive form of this inhibitor protein E3 of BCV was identified as esterase (Vlasak et al., 1988b). The same glycoprotein has been shown previously to be involved in the hemagglutinating activity of BCV (King et al., 1985). Therefore, E3 is designated HE.
- Published
- 1990
- Full Text
- View/download PDF
50. Differential Reactivity of Bovine Coronavirus (BCV) and Influenza C Virus with N-Acetyl-9-O-Acetylneuraminic Acid (NEU5,9AC2)-Containing Receptors
- Author
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B Schultze, Hans-Jürgen Gross, Reinhard Brossmer, G. Herrler, and Hans-Dieter Klenk
- Subjects
Hemagglutination ,biology ,Chemistry ,viruses ,virus diseases ,biology.organism_classification ,Virology ,Virus ,Sialic acid ,Agglutination (biology) ,chemistry.chemical_compound ,Mouse hepatitis virus ,Influenza C Virus ,Receptor ,Bovine coronavirus - Abstract
Only little information is available about the initial events in the infectious cycle of coronaviruses. Attachment of strain A59 of mouse hepatitis virus to the cell surface has been shown to be mediated by a protein of about 110 kDalton (Boyle et al., 1988). Recently, bovine Coronavirus (BCV) and human corona-virus OC43 (HCV-OC43) have been shown to recognize receptors on erythrocytes similar to influenza C virus. The evidence is based on the finding that both influenza C virus and BCV contain a sialate O-acetylesterase, which functions as a receptor-destroying enzyme (Vlasak et al, 1988). Incubation of chicken red blood cells with the esterase of either virus renders the erythrocytes resistant to agglutination by both viruses as well as by HCV-OC43. This result indicates that N-acetyl-9-O-acetylneuraminic acid (Neu5,9Ac2) is a receptor determinant for attachment of BCV and HCV-OC43 to erythrocytes as has been shown previously for influenza C virus (Rogers et al., 1986). Here we confirm the importance of Neu5,9Ac2 for the binding of BCV to the cell surface by resialylation of erythrocytes. We present evidence that strain Johannesburg/1/66 of influenza C virus is more efficient in recognizing Neu5,9Ac2-containing receptors than BCV.
- Published
- 1990
- Full Text
- View/download PDF
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