GLORIA — GEOMAR Library Ocean Research Information Access

1

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AKI - human studies

Kutlay, S. ; Kurultak, I. ; Nergizoglu, G. ; [et al.]

Oxford University Press (OUP) ; 2013

In: Nephrology Dialysis Transplantation Vol. 28, No. suppl 1 ( 2013-05-01), p. i331-i351

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In: Nephrology Dialysis Transplantation, Oxford University Press (OUP), Vol. 28, No. suppl 1 ( 2013-05-01), p. i331-i351

Type of Medium: Online Resource

ISSN: 0931-0509 , 1460-2385

URL: Article

DOI: 10.1093/ndt/gft129

Language: English

Publisher: Oxford University Press (OUP)

Publication Date: 2013

detail.hit.zdb_id: 1465709-0

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2

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Detection of Norwalk virus in stool specimens by reverse transcriptase-polymerase chain reaction and nonradioactive oligoprobes

De Leon, R ; Matsui, S M ; Baric, R S ; [et al.]

American Society for Microbiology ; 1992

In: Journal of Clinical Microbiology Vol. 30, No. 12 ( 1992-12), p. 3151-3157

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In: Journal of Clinical Microbiology, American Society for Microbiology, Vol. 30, No. 12 ( 1992-12), p. 3151-3157

Abstract: A reverse transcriptase (RT)-polymerase chain reaction (PCR)-oligoprobe (OP), or RT-PCR-OP, method was developed for the detection of the Norwalk virus, which causes acute, epidemic gastroenteritis, in stool specimens. The Norwalk virus genome regions encoding the following two proteins were amplified by RT-PCR: the RNA polymerase (260-bp product) and a putative immunogenic protein (224-bp product). The resulting DNA fragments (amplicons) were hybridized to a digoxigenin-labeled internal OP specific to each amplicon. The detection limit of Norwalk virus, as determined by the endpoint of RT-PCR amplification for serially diluted, positive stool specimens, was similar to the actual virion titer as estimated by electron microscopy and at least 100-fold greater than the titer determined by radioimmunoassay (RIA). The RT-PCR-OP assay was specific for Norwalk virus and negative for other enteric viruses, including human and animal caliciviruses, hepatitis E virus, Snow Mountain agent, astroviruses, 16 human enteroviruses, and 5 human rotaviruses. Components of fecal specimens that interfere with RT-PCR were removed successfully by Sephadex G-200 gel chromatography. Of 20 stool specimens from human volunteers that were positive for Norwalk virus by RIA, a specific RT-PCR-OP result was obtained in 95% (19 of 20) of the samples by using the immunogenic protein primers and 75% (15 of 20) by using the polymerase primers. Twenty-six stool specimens from asymptomatic children and adults were negative by the Norwalk virus RT-PCR-OP. RT-PCR-OP detected Norwalk virus in the 4 of 21 coded fecal specimens that were also positive by enzyme immunoassay. Two samples that were positive by RIA or enzyme immunoassay were negative by RT-PCR, perhaps because viral RNA was not present or RT-PCR inhibitors were not adequately removed.

Type of Medium: Online Resource

ISSN: 0095-1137 , 1098-660X

URL: Article

DOI: 10.1128/jcm.30.12.3151-3157.1992

RVK:

XA 10000

Language: English

Publisher: American Society for Microbiology

Publication Date: 1992

detail.hit.zdb_id: 1498353-9

SSG: 12

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3

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Further Evidence for Bats as the Evolutionary Source of Middle East Respiratory Syndrome Coronavirus

Anthony, S. J. ; Gilardi, K. ; Menachery, V. D. ; [et al.]

American Society for Microbiology ; 2017

In: mBio Vol. 8, No. 2 ( 2017-05-03)

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In: mBio, American Society for Microbiology, Vol. 8, No. 2 ( 2017-05-03)

Abstract: Global surveillance efforts for undiscovered viruses are an important component of pandemic prevention initiatives. These surveys can be useful for finding novel viruses and for gaining insights into the ecological and evolutionary factors driving viral diversity; however, finding a viral sequence is not sufficient to determine whether it can infect people (i.e., poses a zoonotic threat). Here, we investigated the specific zoonotic risk of a MERS-like coronavirus (PREDICT/PDF-2180) identified in a bat from Uganda and showed that, despite being closely related to MERS-CoV, it is unlikely to pose a threat to humans. We suggest that this approach constitutes an appropriate strategy for beginning to determine the zoonotic potential of wildlife viruses. By showing that PREDICT/PDF-2180 does not infect cells that express the functional receptor for MERS-CoV, we further show that recombination was likely to be the critical step that allowed MERS to emerge in humans.

Type of Medium: Online Resource

ISSN: 2161-2129 , 2150-7511

URL: Article

DOI: 10.1128/mBio.00373-17

Language: English

Publisher: American Society for Microbiology

Publication Date: 2017

detail.hit.zdb_id: 2557172-2

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4

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Characterization of leader RNA sequences on the virion and mRNAs of mouse hepatitis virus, a cytoplasmic RNA virus.

Lai, M M ; Baric, R S ; Brayton, P R ; [et al.]

Proceedings of the National Academy of Sciences ; 1984

In: Proceedings of the National Academy of Sciences Vol. 81, No. 12 ( 1984-06), p. 3626-3630

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In: Proceedings of the National Academy of Sciences, Proceedings of the National Academy of Sciences, Vol. 81, No. 12 ( 1984-06), p. 3626-3630

Abstract: Mouse hepatitis virus, which replicates in cytoplasm, contains leader RNA sequences at the 5' end of the virus-specific mRNAs. We have sequenced this leader RNA by synthesizing cDNA from a synthetic oligodeoxyribonucleotide primer (15-mer) that is complementary to the sequences at the junction site between the leader and body sequences of the mRNAs. The leader sequences on each mRNA have exactly the same size, which span approximately equal to 70 nucleotides. Leader cDNA fragments obtained from several mRNA species were sequenced and found to be identical. Computer analysis of the leader RNA sequences shows that they share extensive sequence homology with the long-terminal-repeat region of several mammalian sarcoma viruses, suggesting possible common functions. This is a novel case of spliced leader sequences in the mRNAs of a cytoplasmic virus. An identical leader sequence is also present at the 5' end of the virion genomic RNA. The leader RNA is thus probably encoded by the virion genomic RNA template and is fused to the different body sequences of the various mRNAs. Since conventional RNA splicing is not involved, a novel mechanism for fusing two noncontiguous RNA segments in the cytoplasm must be utilized during viral transcription. Several minor cDNA bands longer than the leader were also synthesized, suggesting the possible presence of partially homologous sequences in other parts of the genome RNA.

Type of Medium: Online Resource

ISSN: 0027-8424 , 1091-6490

URL: Article

DOI: 10.1073/pnas.81.12.3626

RVK:

TA 1000

RVK:

WA 15000

Language: English

Publisher: Proceedings of the National Academy of Sciences

Publication Date: 1984

detail.hit.zdb_id: 209104-5

detail.hit.zdb_id: 1461794-8

SSG: 11

SSG: 12

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5

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Specific interaction between coronavirus leader RNA and nucleocapsid protein

Stohlman, S A ; Baric, R S ; Nelson, G N ; [et al.]

American Society for Microbiology ; 1988

In: Journal of Virology Vol. 62, No. 11 ( 1988-11), p. 4288-4295

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In: Journal of Virology, American Society for Microbiology, Vol. 62, No. 11 ( 1988-11), p. 4288-4295

Abstract: Northwestern blot analysis in the presence of competitor RNA was used to examine the interaction between the mouse hepatitis virus (MHV) nucleocapsid protein (N) and virus-specific RNAs. Our accompanying article demonstrates that anti-N monoclonal antibodies immunoprecipitated all seven MHV-specific RNAs as well as the small leader-containing RNAs from infected cells. In this article we report that a Northwestern blotting protocol using radiolabeled viral RNAs in the presence of host cell competitor RNA can be used to demonstrate a high-affinity interaction between the MHV N protein and the virus-specific RNAs. Further, RNA probes prepared by in vitro transcription were used to define the sequences that participate in such high-affinity binding. A specific interaction occurs between the N protein and sequences contained with the leader RNA which is conserved at the 5' end of all MHV RNAs. We have further defined the binding sites to the area of nucleotides 56 to 65 at the 3' end of the leader RNA and suggest that this interaction may play an important role in the discontinuous nonprocessive RNA transcriptional process unique to coronaviruses.

Type of Medium: Online Resource

ISSN: 0022-538X , 1098-5514

URL: Article

DOI: 10.1128/jvi.62.11.4288-4295.1988

Language: English

Publisher: American Society for Microbiology

Publication Date: 1988

detail.hit.zdb_id: 1495529-5

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6

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Interactions between coronavirus nucleocapsid protein and viral RNAs: implications for viral transcription

Baric, R S ; Nelson, G W ; Fleming, J O ; [et al.]

American Society for Microbiology ; 1988

In: Journal of Virology Vol. 62, No. 11 ( 1988-11), p. 4280-4287

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In: Journal of Virology, American Society for Microbiology, Vol. 62, No. 11 ( 1988-11), p. 4280-4287

Abstract: The interaction of the mouse hepatitis virus (MHV) nucleocapsid protein (N) and viral RNA was examined. Monoclonal antibody specific for N protein coimmunoprecipitated MHV genomic RNA as well as all six MHV subgenomic mRNAs found in MHV-infected cells. In contrast, monoclonal antibodies to the MHV E2 or E1 envelope glycoproteins, an anti-I-A monoclonal antibody, and serum samples from lupus patients did not immunoprecipitate the MHV mRNAs. Moreover, the anti-N monoclonal antibody did not coimmunoprecipitate vesicular stomatitis virus RNA or host cell RNA under conditions which immunoprecipitated all MHV RNAs. These data suggest a specific interaction between the N protein and the virus-specific mRNAs. Both the membrane-bound and cytosolic small MHV leader-specific RNAs of greater than 65 nucleotides long were immunoprecipitated only by anti-N monoclonal antibody. These data suggest that an N binding site is present within the leader RNA sequences at a site at least 65 nucleotides from the 5' end of genomic RNA and all six subgenomic mRNAs. The larger leader-containing RNAs originating from mRNA 1 and mRNA 6, as well as the MHV negative-stranded RNA, were also immunoprecipitated by the anti-N monoclonal antibody. These data indicate that the MHV N protein is associated with MHV-specific RNAs and RNA intermediates and may play an important functional role during MHV transcription and replication.

Type of Medium: Online Resource

ISSN: 0022-538X , 1098-5514

URL: Article

DOI: 10.1128/jvi.62.11.4280-4287.1988

Language: English

Publisher: American Society for Microbiology

Publication Date: 1988

detail.hit.zdb_id: 1495529-5

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7

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Recombination between nonsegmented RNA genomes of murine coronaviruses

Lai, M M ; Baric, R S ; Makino, S ; [et al.]

American Society for Microbiology ; 1985

In: Journal of Virology Vol. 56, No. 2 ( 1985-11), p. 449-456

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In: Journal of Virology, American Society for Microbiology, Vol. 56, No. 2 ( 1985-11), p. 449-456

Abstract: We have isolated a recombinant virus between the A59 and JHM strains of mouse hepatitis virus, which contain a single species of nonsegmented RNA genome. This recombinant was derived by mixed infection of DBT cells with temperature-sensitive mutants of A59 and JHM at nonpermissive temperature. Viruses recovered at this temperature were screened by oligonucleotide fingerprinting of their genomic RNAs. One recombinant virus, B1, was found to contain mostly A59-derived sequences, but the 3 kilobases at the 5' end of the genomic RNA was derived from JHM. Thus, the crossover point in the B1 genome is located within gene A, which codes for the viral RNA polymerases. The study of the intracellular RNA species of B1 virus revealed that probably all of the virus-specific subgenomic mRNA species contained the body sequences of strain A59 but the leader sequences of JHM. This result indicates that the JHM leader RNA, which differs from the A59 leader RNA, could be fused to the mRNAs of a different virus strain during RNA transcription. Furthermore, B1 virus-infected cells contain an additional subgenomic mRNA species which is transcribed from a new initiation site within gene C, suggesting that the leader RNA could determine the site of initiation for coronavirus mRNAs. These data represent a first report of RNA recombination between viruses, other than picornaviruses, which contain nonsegmented RNA genomes.

Type of Medium: Online Resource

ISSN: 0022-538X , 1098-5514

URL: Article

DOI: 10.1128/jvi.56.2.449-456.1985

Language: English

Publisher: American Society for Microbiology

Publication Date: 1985

detail.hit.zdb_id: 1495529-5

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8

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Reduced synthesis of Sindbis virus negative strand RNA in cultures treated with host transcription inhibitors

Baric, R S ; Lineberger, D W ; Johnston, R E

American Society for Microbiology ; 1983

In: Journal of Virology Vol. 47, No. 1 ( 1983-07), p. 46-54

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In: Journal of Virology, American Society for Microbiology, Vol. 47, No. 1 ( 1983-07), p. 46-54

Abstract: Host cell involvement in Sindbis virus (SB) RNA synthesis was examined in cells which had been treated before infection with actinomycin D or alpha-amanitin (alpha-A). Overall synthesis of SB RNA was reduced significantly in CHO cells treated for 18 h before infection with alpha-A. However, SB RNA was produced at near normal levels in CHOama-1 cells, a line which contains an alpha-A-resistant RNA polymerase II. In BHK or CHO cells infected with SBamr, a mutant which replicates normally in cells pretreated with either actinomycin D or alpha-A, viral RNA synthesis was not decreased. The levels of negative strand RNA and of replicative forms I, II, and III in SB-infected cells were progressively reduced with increasing times of pretreatment with host transcription inhibitors, indicating fewer functional replicative intermediates in treated cells. Replicative events after replicative intermediate formation also were inhibited but only to the extent predicted by the reduction in replicative intermediates. Similarly, events preceding negative strand synthesis, adsorption, penetration, uncoating, and translation of nonstructural proteins, apparently were not impeded in treated cells. Therefore, our results are consistent with the involvement of a host component after translation of the nonstructural proteins but before or during the synthesis of SB negative strand RNA.

Type of Medium: Online Resource

ISSN: 0022-538X , 1098-5514

URL: Article

DOI: 10.1128/jvi.47.1.46-54.1983

Language: English

Publisher: American Society for Microbiology

Publication Date: 1983

detail.hit.zdb_id: 1495529-5

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9

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Detection of low levels of enteric viruses in metropolitan and airplane sewage

Shieh, Y S ; Baric, R S ; Sobsey, M D

American Society for Microbiology ; 1997

In: Applied and Environmental Microbiology Vol. 63, No. 11 ( 1997-11), p. 4401-4407

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In: Applied and Environmental Microbiology, American Society for Microbiology, Vol. 63, No. 11 ( 1997-11), p. 4401-4407

Abstract: To detect less prevalent viruses, such as wild-type polioviruses in sewage from a highly immunized community, a method was developed to efficiently recover viruses and remove PCR inhibitors. The method consisted of initial separation of solids from liquid, followed by solvent extractions, polyethylene glycol precipitations, Sephadex G-200 chromatography, and guanidinium isothiocyanate (GIT) extraction. To elute viruses from the separated solids, 0.5 M threonine (pH 7.5) was as efficient as 3% beef extract but conferred no PCR inhibition. In samples that were concentrated approximately 1,000-fold, 21% of the initially seeded viruses were recovered. When poliovirus type 3 (PV3) Sabin strain at low levels and PV1 LSc strain at high levels were seeded in raw sewage, PV3 was specifically detected in the final sample concentrates at sensitivities of 14 PFU by direct PCR and 0.7 PFU by GIT extraction-PCR. While applying the method to international airplane sewage, which contains high levels of solids as well as commercial sanitizers, 44% (7 of 16) of the samples were found to harbor enteroviruses by both cell culture infectivity and pan-enterovirus PCR analyses. Nucleotide sequencing of the PCR products revealed that multiple enterovirus genotypes were amplified from each final sewage concentrate, whereas the fewer virus genotypes detected by cell culture infectivity were probably the better growing strains. By this method, we demonstrated that air travel may contribute to the intercontinental dissemination of enteric pathogens.

Type of Medium: Online Resource

ISSN: 0099-2240 , 1098-5336

URL: Article

DOI: 10.1128/aem.63.11.4401-4407.1997

RVK:

WA 15000

Language: English

Publisher: American Society for Microbiology

Publication Date: 1997

detail.hit.zdb_id: 223011-2

detail.hit.zdb_id: 1478346-0

SSG: 12

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10

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Presence of leader sequences in the mRNA of mouse hepatitis virus

Lai, M M ; Patton, C D ; Baric, R S ; [et al.]

American Society for Microbiology ; 1983

In: Journal of Virology Vol. 46, No. 3 ( 1983-06), p. 1027-1033

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In: Journal of Virology, American Society for Microbiology, Vol. 46, No. 3 ( 1983-06), p. 1027-1033

Abstract: To determine the structure and the mechanism of synthesis of mouse hepatitis virus mRNA, the map positions of the large RNase T1-resistant oligonucleotides of the seven mouse hepatitis virus strain A59 intracellular mRNA species were studied. We found that all but one of the oligonucleotides were mapped at the positions within each mRNA consistent with the nested-set, stairlike structure of mouse hepatitis virus mRNA (Lai et al., J. Virol. 39:823-834). However, one oligonucleotide, 10, was mapped near the 5' ends of every mRNA and virion genomic RNA. In other words, oligonucleotide 10 and, therefore, the sequences around the 5' ends of the mRNAs are not colinear with the genomic sequences. Because this oligonucleotide is present only once in the genomic RNA, this result indicates that oligonucleotide 10 is not transcribed from multiple sites on the genomic template, but rather represents a leader RNA sequence which is joined to the body sequences of the different mRNAs during mRNA transcription. This provides the most direct evidence thus far for the presence of leader sequences in the mRNAs of mouse hepatitis virus, which is a cytoplasmic virus. Several possible mechanisms of RNA synthesis are discussed.

Type of Medium: Online Resource

ISSN: 0022-538X , 1098-5514

URL: Article

DOI: 10.1128/jvi.46.3.1027-1033.1983

Language: English

Publisher: American Society for Microbiology

Publication Date: 1983

detail.hit.zdb_id: 1495529-5

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