22 results on '"Binger, Tabea"'
Search Results
2. Genetic characterization of varicella-zoster and HIV-1 viruses from the cerebrospinal fluid of a co-infected encephalitic patient, Ghana
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El-Duah, Philip, Sylverken, Augustina Angelina, Owusu, Michael, Amoako, Yaw Ampem, Yeboah, Richmond, Gorman, Richmond, Nyarko-Afriyie, Emmanuella, Schneider, Julia, Jones, Terry C., Bonney, Joseph, Adade, Titus, Yeboah, Eric Smart, Binger, Tabea, Corman, Victor Max, Drosten, Christian, and Phillips, Richard Odame
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- 2022
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3. Transmission of SARS-CoV-2 in northern Ghana: insights from whole-genome sequencing
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Sylverken, Augustina Angelina, El-Duah, Philip, Owusu, Michael, Schneider, Julia, Yeboah, Richmond, Ayisi-Boateng, Nana Kwame, Gorman, Richmond, Adu, Eric, Kwarteng, Alexander, Frimpong, Michael, Binger, Tabea, Aryeetey, Sherihane, Asamoah, Jesse Addo, Amoako, Yaw Ampem, Amuasi, John Humphrey, Beheim-Schwarzbach, Jörn, Owusu-Dabo, Ellis, Adu-Sarkodie, Yaw, Obiri-Danso, Kwasi, Corman, Victor Max, Drosten, Christian, and Phillips, Richard
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- 2021
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4. Detection and genomic characterization of hepatitis E virus genotype 3 from pigs in Ghana, Africa
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El-Duah, Philip, Dei, Dickson, Binger, Tabea, Sylverken, Augustina, Wollny, Robert, Tasiame, William, Oppong, Samuel, Adu-Sarkodie, Yaw, Emikpe, Benjamin, Folitse, Raphael, Drexler, Jan Felix, Phillips, Richard, Drosten, Christian, and Corman, Victor Max
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- 2020
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5. Viral Shedding and Antibody Response in 37 Patients With Middle East Respiratory Syndrome Coronavirus Infection
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Corman, Victor M., Albarrak, Ali M., Omrani, Ali Senosi, Albarrak, Mohammed M., Farah, Mohamed Elamin, Almasri, Malak, Muth, Doreen, Sieberg, Andrea, Meyer, Benjamin, Assiri, Abdullah M., Binger, Tabea, Steinhagen, Katja, Lattwein, Erik, Al-Tawfiq, Jaffar, Müller, Marcel A., Drosten, Christian, and Memish, Ziad A.
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- 2016
6. Fusion activity of African henipavirus F proteins with a naturally occurring start codon directly upstream of the signal peptide
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Weis, Michael, Behner, Laura, Binger, Tabea, Drexler, Jan Felix, Drosten, Christian, and Maisner, Andrea
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- 2015
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7. Attenuation of replication by a 29 nucleotide deletion in SARS-coronavirus acquired during the early stages of human-to-human transmission
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Muth, Doreen, Corman, Victor Max, Roth, Hanna, Binger, Tabea, Dijkman, Ronald, Gottula, Lina Theresa, Gloza-Rausch, Florian, Balboni, Andrea, Battilani, Mara, Rihtarič, Danijela, Toplak, Ivan, Ameneiros, Ramón Seage, Pfeifer, Alexander, Thiel, Volker, Drexler, Jan Felix, Müller, Marcel Alexander, and Drosten, Christian
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- 2018
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8. Bats carry pathogenic hepadnaviruses antigenically related to hepatitis B virus and capable of infecting human hepatocytes
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Drexler, Jan Felix, Geipel, Andreas, König, Alexander, Corman, Victor M., van Riel, Debby, Leijten, Lonneke M., Bremer, Corinna M., Rasche, Andrea, Cottontail, Veronika M., Magangaf, Gael D., Schlegel, Mathias, Müller, Marcel A., Adam, Alexander, Klose, Stefan M., Carneiro, Aroldo José Borges, Stöcker, Andreas, Franke, Carlos Roberto, Rausch, Florian Gloza, Geyer, Joachim, Annan, Augustina, Adu-Sarkodie, Yaw, Oppongn, Samuel, Binger, Tabea, Vallo, Peter, Tschapka, Marco, Ulrich, Rainer G., Gerlich, Wolfram H., Leroy, Eric, Kuiken, Thijs, Glebe, Dieter, and Drosten, Christian
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- 2013
9. Migration potential and gene expression profile of human mesenchymal stem cells induced by CCL25
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Binger, Tabea, Stich, Stefan, Andreas, Kristin, Kaps, Christian, Sezer, Orhan, Notter, Michael, Sittinger, Michael, and Ringe, Jochen
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- 2009
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10. Epidemiological profile of SARS-CoV-2 among selected regions in Ghana: A cross-sectional retrospective study.
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Owusu, Michael, Sylverken, Augustina Angelina, Ankrah, Sampson Twumasi, El-Duah, Philip, Ayisi-Boateng, Nana Kwame, Yeboah, Richmond, Gorman, Richmond, Asamoah, Jesse, Binger, Tabea, Acheampong, Godfred, Bekoe, Franklin Asiedu, Ohene, Sally-Ann, Larsen-Reindorf, Rita, Awuah, Anthony Afum-Adjei, Amuasi, John, Owusu-Dabo, Ellis, Adu-Sarkodie, Yaw, and Phillips, Richard Odame
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CROSS-sectional method ,SARS-CoV-2 ,REVERSE transcriptase polymerase chain reaction ,MEDICAL personnel - Abstract
Background: Global cases of COVID-19 continue to rise, causing havoc to several economies. So far, Ghana has recorded 48,643 confirmed cases with 320 associated deaths. Although summaries of data are usually provided by the Ministry of Health, detailed epidemiological profile of cases are limited. This study sought to describe the socio-demographic features, pattern of COVID-19 spread and the viral load dynamics among subjects residing in northern, middle and part of the southern belt of Ghana. Methods: This was a cross-sectional retrospective study that reviewed records of samples collected from February to July, 2020. Respiratory specimens such as sputum, deep-cough saliva and nasopharyngeal swabs were collected from suspected COVID-19 subjects in 12 regions of Ghana for laboratory analysis and confirmation by real-time reverse transcription polymerase chain reaction (RT-PCR). Results: A total of 72,434 samples were collected during the review period, with majority of the sampled individuals being females (37,464; 51.9%). The prevalence of SARS-CoV-2 identified in the study population was 13.2% [95%CI: 12.9, 13.4). Males were mostly infected (4,897; 51.5%) compared to females. Individuals between the ages 21–30 years recorded the highest number of infections (3,144, 33.4%). Symptomatic subjects had higher viral loads (1479.7 copies/μl; IQR = 40.6–178919) than asymptomatic subjects (49.9; IQR = 5.5–3641.6). There was significant association between gender or age and infection with SARS-CoV-2 (p<0.05). Among all the suspected clinical presentations, anosmia was the strongest predictor of SARS-CoV-2 infection (Adj. OR (95%CI): 24.39 (20.18, 29.49). We observed an average reproductive number of 1.36 with a minimum of 1.28 and maximum of 1.43. The virus trajectory shows a gradual reduction of the virus reproductive number. Conclusion: This study has described the epidemiological profile of COVID-19 cases in northern, middle and part of the southern belt of Ghana, with males and younger individuals at greater risk of contracting the disease. Health professionals should be conscious of individuals presenting with anosmia since this was seen as the strongest predictor of virus infection. [ABSTRACT FROM AUTHOR]
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- 2020
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11. Diagnostics for COVID-19: A case for field-deployable, rapid molecular tests for community surveillance.
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Frimpong, Michael, Amoako, Yaw A., Anim, Kwadwo B., Ahor, Hubert S., Yeboah, Richmond, Arthur, Joshua, Dakorah, Justin S., Gborgblovor, Delphine, Akrofi, Samuel, Sekyi-Djan, Phyllis, Owusu, Michael, Sylverken, Augustina A., Binger, Tabea, and Phillips, Richard O.
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COVID-19 ,SARS-CoV-2 ,COVID-19 pandemic ,CONTACT tracing ,VIRAL transmission - Abstract
Across the globe, the outbreak of the COVID-19 pandemic is causing distress with governments doing everything in their power to contain the spread of the novel coronavirus (SARS-CoV-2) to prevent morbidity and mortality. Actions are being implemented to keep health care systems from being overstretched and to curb the outbreak. Any policy responses aimed at slowing down the spread of the virus and mitigating its immediate effects on health care systems require a firm basis of information about the absolute number of currently infected people, growth rates, and locations/hotspots of infections. The only way to obtain this base of information is by conducting numerous tests in a targeted way. Currently, in Ghana, there is a centralized testing approach, that takes 4-5 days for samples to be shipped and tested at central reference laboratories with results communicated to the district, regional and national stakeholders. This delay in diagnosis increases the risk of ongoing transmission in communities and vulnerable institutions. We have validated, evaluated and deployed an innovative diagnostic tool on a mobile laboratory platform to accelerate the COVID-19 testing. A preliminary result of 74 samples from COVID-19 suspected cases has a positivity rate of 12% with a turn-around time of fewer than 3 hours from sample taking to reporting of results, significantly reducing the waiting time from days to hours, enabling expedient response by the health system for contact tracing to reduce transmission and additionally improving case management. [ABSTRACT FROM AUTHOR]
- Published
- 2020
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12. Burden of influenza among hospitalized febrile children in Ghana.
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Hogan, Benedikt, Ammer, Luise, Zimmermann, Marlow, Binger, Tabea, Krumkamp, Ralf, Sarpong, Nimako, Rettig, Theresa, Dekker, Denise, Kreuels, Benno, Reigl, Lisa, Boahen, Kennedy G., Wiafe, Charity, Adu‐Sarkodie, Yaw, Owusu‐Dabo, Ellis, May, Jürgen, and Eibach, Daniel
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INFLUENZA diagnosis ,INFLUENZA treatment ,HOSPITAL care ,CHILDREN ,RURAL health - Abstract
Background Influenza surveillance data from Africa indicate a substantial disease burden with high mortality. However, local influenza data from district hospitals with limited laboratory facilities are still scarce. Objectives To identify the frequency and seasonal distribution of influenza among hospitalized febrile children in a rural hospital in Ghana and to describe differential diagnoses to other severe febrile infections. Methods Between January 2014 and April 2015, all children with a temperature of ≥38°C admitted to a district hospital in Ghana were screened for influenza A and B by RT- PCR and differentiated to subtypes A(H1N1)pdm09 and A(H3N2). Malaria microscopy and blood cultures were performed for each patient. Results A total of 1063 children with a median age of 2 years ( IQR: 1-4 years) were recruited. Of those, 271 (21%) were classified as severe acute respiratory infection ( SARI) and 47 (4%) were positive for influenza, namely 26 (55%) influenza B, 15 (32%) A(H1N1)pdm09, and 6 (13%) A(H3N2) cases. Influenza predominantly occurred in children aged 3-5 years and was more frequently detected in the major rainy season ( OR = 2.9; 95% CI: 1.47-6.19) during the first half of the year. Two (4%) and seven (15%) influenza-positive children were co-diagnosed with an invasive bloodstream infection or malaria, respectively. Conclusion Influenza contributes substantially to the burden of hospitalized febrile children in Ghana being strongly dependent on age and corresponds with the major rainy season during the first half-year. [ABSTRACT FROM AUTHOR]
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- 2017
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13. Viral Shedding and Antibody Response in 37 PatientsWith Middle East Respiratory Syndrome Coronavirus Infection.
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Corman, Victor M., Albarrak, Ali M., Omrani, Ali Senosi, Albarrak, Mohammed M., Farah, Mohamed Elamin, Almasri, Malak, Muth, Doreen, Sieberg, Andrea, Meyer, Benjamin, Assiri, Abdullah M., Binger, Tabea, Steinhagen, Katja, Lattwein, Erik, Al-Tawfiq, Jaffar, Müller, Marcel A., Drosten, Christian, and Memish, Ziad A.
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VIRAL shedding ,ANTIBODY formation ,MIDDLE East respiratory syndrome ,MERS coronavirus ,IMMUNOGLOBULIN M ,DIAGNOSIS - Abstract
Background. The Middle East respiratory syndrome (MERS) coronavirus causes isolated cases and outbreaks of severe respiratory disease. Essential features of the natural history of disease are poorly understood. Methods. We studied 37 adult patients infected with MERS coronavirus for viral load in the lower and upper respiratory tracts (LRT and URT, respectively), blood, stool, and urine. Antibodies and serum neutralizing activities were determined over the course of disease. Results. One hundred ninety-nine LRT samples collected during the 3 weeks following diagnosis yielded virus RNA in 93% of tests. Average (maximum) viral loads were 5 × 10
6 (6 × 1010 ) copies/mL. Viral loads ( positive detection frequencies) in 84 URT samples were 1.9 × 104 copies/mL (47.6%). Thirty-three percent of all 108 serum samples tested yielded viral RNA. Only 14.6% of stool and 2.4% of urine samples yielded viral RNA. All seroconversions occurred during the first 2 weeks after diagnosis, which corresponds to the second and third week after symptom onset. Immunoglobulin M detection provided no advantage in sensitivity over immunoglobulin G (IgG) detection. All surviving patients, but only slightly more than half of all fatal cases, produced IgG and neutralizing antibodies. The levels of IgG and neutralizing antibodies were weakly and inversely correlated with LRT viral loads. Presence of antibodies did not lead to the elimination of virus from LRT. Conclusions. The timing and intensity of respiratory viral shedding in patients with MERS closely matches that of those with severe acute respiratory syndrome. Blood viral RNA does not seem to be infectious. Extrapulmonary loci of virus replication seem possible. Neutralizing antibodies do not suffice to clear the infection. [ABSTRACT FROM AUTHOR]- Published
- 2016
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14. Lagos bat virus transmission in an Eidolon helvum bat colony, Ghana.
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Freuling, Conrad M., Binger, Tabea, Beer, Martin, Adu-Sarkodie, Yaw, Schatz, Juliane, Fischer, Melina, Hanke, Dennis, Hoffmann, Bernd, Höper, Dirk, Mettenleiter, Thomas C., Oppong, Samual K., Drosten, Christian, and Müller, Thomas
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BAT diseases , *VIRUS disease transmission , *STRAW-colored fruit bat , *LYSSAVIRUS - Abstract
A brain sample of a straw-coloured fruit bat ( Eidolon helvum ) from Ghana without evident signs of disease tested positive by generic Lyssavirus RT-PCR and direct antigen staining. Sequence analysis confirmed the presence of a Lagos bat virus belonging to phylogenetic lineage A. Virus neutralization tests using the isolate with sera from the same group of bats yielded neutralizing antibodies in 74% of 567 animals. No cross-neutralization was observed against a different Lagos bat virus (lineage B). [ABSTRACT FROM AUTHOR]
- Published
- 2015
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15. Filovirus receptor NPC1 contributes to species-specific patterns of ebolavirus susceptibility in bats.
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Melinda Ng, Ndungo, Esther, Kaczmarek, Maria E., Herbert, Andrew S., Binger, Tabea, Kuehne, Ana I., Jangra, Rohit K., Hawkins, John A., Gifford, Robert J., Biswas, Rohan, Demogines, Ann, James, Rebekah M., Meng Yu, Brummelkamp, Thijn R., Drosten, Christian, Lin-Fa Wang, Kuhn, Jens H., Müller, Marcel A., Dye, John M., and Sawyer, Sara L.
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- 2015
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16. Serological Evidence of Influenza A Viruses in Frugivorous Bats from Africa.
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Freidl, Gudrun Stephanie, Binger, Tabea, Müller, Marcel Alexander, de Bruin, Erwin, van Beek, Janko, Corman, Victor Max, Rasche, Andrea, Drexler, Jan Felix, Sylverken, Augustina, Oppong, Samuel K., Adu-Sarkodie, Yaw, Tschapka, Marco, Cottontail, Veronika M., Drosten, Christian, and Koopmans, Marion
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INFLUENZA A virus , *SEROLOGY , *FRUGIVORES , *BATS , *ZOONOSES , *EBOLA virus , *VIRAL ecology - Abstract
Bats are likely natural hosts for a range of zoonotic viruses such as Marburg, Ebola, Rabies, as well as for various Corona- and Paramyxoviruses. In 2009/10, researchers discovered RNA of two novel influenza virus subtypes – H17N10 and H18N11 – in Central and South American fruit bats. The identification of bats as possible additional reservoir for influenza A viruses raises questions about the role of this mammalian taxon in influenza A virus ecology and possible public health relevance. As molecular testing can be limited by a short time window in which the virus is present, serological testing provides information about past infections and virus spread in populations after the virus has been cleared. This study aimed at screening available sera from 100 free-ranging, frugivorous bats (Eidolon helvum) sampled in 2009/10 in Ghana, for the presence of antibodies against the complete panel of influenza A haemagglutinin (HA) types ranging from H1 to H18 by means of a protein microarray platform. This technique enables simultaneous serological testing against multiple recombinant HA-types in 5μl of serum. Preliminary results indicate serological evidence against avian influenza subtype H9 in about 30% of the animals screened, with low-level cross-reactivity to phylogenetically closely related subtypes H8 and H12. To our knowledge, this is the first report of serological evidence of influenza A viruses other than H17 and H18 in bats. As avian influenza subtype H9 is associated with human infections, the implications of our findings from a public health context remain to be investigated. [ABSTRACT FROM AUTHOR]
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- 2015
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17. A Novel Rhabdovirus Isolated from the Straw-Colored Fruit Bat Eidolon helvum, with Signs of Antibodies in Swine and Humans.
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Binger, Tabea, Annan, Augustina, Drexler, Jan Felix, Müller, Marcel Alexander, Kallies, René, Adankwah, Ernest, Wollny, Robert, Kopp, Anne, Heidemann, Hanna, Dei, Dickson, Agya-Yao, Festus Courage, Junglen, Sandra, Feldt, Torsten, Kurth, Andreas, Oppong, Samuel, Adu-Sarkodie, Yaw, and Drosten, Christian
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BATS , *VIRUSES , *RHABDOVIRUSES , *DISEASE prevalence , *IMMUNOFLUORESCENCE - Abstract
Bats have been implicated as reservoirs of emerging viruses. Bat species forming large social groups and roosting in proximity to human communities are of particular interest. In this study, we sampled a colony of ca. 350,000 individuals of the straw-colored fruit bat Eidolon helvum in Kumasi, the second largest city of Ghana. A novel rhabdovirus (Kumasi rhabdovirus [KRV]) was isolated in E. helvum cell cultures and passaged to Vero cells as well as interferon-competent human and primate cells (A549 and MA104). Genome composition was typical for a rhabdovirus. KRV was detected in 5.1% of 487 animals, showing association with the spleen but not the brain. Antibody prevalence was 11.5% by immunofluorescence and 6.4% by plaque reduction virus neutralization test (PRNT). Detection throughout 3 sampling years was pronounced in both annual wet seasons, of which only one overlaps the postparturition season. Juvenile bats showed increased viral prevalence. No evidence of infection was obtained in 1,240 female mosquitos (6 different genera) trapped in proximity to the colony to investigate potential vector association. Antibodies were found in 28.9% (5.4% by PRNT) of 107 swine sera but not in similarly large collections of sheep, goat, or cattle sera. The antibody detection rate in human subjects with occupational exposure to the bat colony was 11% (5/45 persons), which was significantly higher than in unexposed adults (0.8% [1/118]; chi square, P<0.001). KRV is a novel bat-associated rhabdovirus potentially transmitted to humans and swine. Disease associations should be investigated. [ABSTRACT FROM AUTHOR]
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- 2015
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18. Differential Sensitivity of Bat Cells to Infection by Enveloped RNA Viruses: Coronaviruses, Paramyxoviruses, Filoviruses, and Influenza Viruses.
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Hoffmann, Markus, Müller, Marcel Alexander, Drexler, Jan Felix, Glende, Jörg, Erdt, Meike, Gützkow, Tim, Losemann, Christoph, Binger, Tabea, Deng, Hongkui, Schwegmann-Weßels, Christel, Esser, Karl-Heinz, Drosten, Christian, and Herrler, Georg
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RNA viruses ,VIRUS diseases ,VIRAL envelopes ,CORONAVIRUSES ,PARAMYXOVIRUSES ,FILOVIRIDAE ,INFLUENZA viruses - Abstract
Bats (Chiroptera) host major human pathogenic viruses including corona-, paramyxo, rhabdo- and filoviruses. We analyzed six different cell lines from either Yinpterochiroptera (including African flying foxes and a rhinolophid bat) or Yangochiroptera (genera Carollia and Tadarida) for susceptibility to infection by different enveloped RNA viruses. None of the cells were sensitive to infection by transmissible gastroenteritis virus (TGEV), a porcine coronavirus, or to infection mediated by the Spike (S) protein of SARS-coronavirus (SARS-CoV) incorporated into pseudotypes based on vesicular stomatitis virus (VSV). The resistance to infection was overcome if cells were transfected to express the respective cellular receptor, porcine aminopeptidase N for TGEV or angiotensin-converting enzyme 2 for SARS-CoV. VSV pseudotypes containing the S proteins of two bat SARS-related CoV (Bg08 and Rp3) were unable to infect any of the six tested bat cell lines. By contrast, viral pseudotypes containing the surface protein GP of Marburg virus from the family Filoviridae infected all six cell lines though at different efficiency. Notably, all cells were sensitive to infection by two paramyxoviruses (Sendai virus and bovine respiratory syncytial virus) and three influenza viruses from different subtypes. These results indicate that bat cells are more resistant to infection by coronaviruses than to infection by paramyxoviruses, filoviruses and influenza viruses. Furthermore, these results show a receptor-dependent restriction of the infection of bat cells by CoV. The implications for the isolation of coronaviruses from bats are discussed. [ABSTRACT FROM AUTHOR]
- Published
- 2013
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19. Evidence for Novel Hepaciviruses in Rodents.
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Drexler, Jan Felix, Corman, Victor Max, Müller, Marcel Alexander, Lukashev, Alexander N., Gmyl, Anatoly, Coutard, Bruno, Adam, Alexander, Ritz, Daniel, Leijten, Lonneke M., van Riel, Debby, Kallies, Rene, Klose, Stefan M., Gloza-Rausch, Florian, Binger, Tabea, Annan, Augustina, Adu-Sarkodie, Yaw, Oppong, Samuel, Bourgarel, Mathieu, Rupp, Daniel, and Hoffmann, Bernd
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HEPATITIS C virus ,CIRRHOSIS of the liver ,LIVER cancer ,LABORATORY rodents ,BLOODBORNE infections - Abstract
Hepatitis C virus (HCV) is among the most relevant causes of liver cirrhosis and hepatocellular carcinoma. Research is complicated by a lack of accessible small animal models. The systematic investigation of viruses of small mammals could guide efforts to establish such models, while providing insight into viral evolutionary biology. We have assembled the so-far largest collection of small-mammal samples from around the world, qualified to be screened for bloodborne viruses, including sera and organs from 4,770 rodents (41 species); and sera from 2,939 bats (51 species). Three highly divergent rodent hepacivirus clades were detected in 27 (1.8%) of 1,465 European bank voles (Myodes glareolus) and 10 (1.9%) of 518 South African four-striped mice (Rhabdomys pumilio). Bats showed anti-HCV immunoblot reactivities but no virus detection, although the genetic relatedness suggested by the serologic results should have enabled RNA detection using the broadly reactive PCR assays developed for this study. 210 horses and 858 cats and dogs were tested, yielding further horse-associated hepaciviruses but none in dogs or cats. The rodent viruses were equidistant to HCV, exceeding by far the diversity of HCV and the canine/equine hepaciviruses taken together. Five full genomes were sequenced, representing all viral lineages. Salient genome features and distance criteria supported classification of all viruses as hepaciviruses. Quantitative RT-PCR, RNA in-situ hybridisation, and histopathology suggested hepatic tropism with liver inflammation resembling hepatitis C. Recombinant serology for two distinct hepacivirus lineages in 97 bank voles identified seroprevalence rates of 8.3 and 12.4%, respectively. Antibodies in bank vole sera neither cross-reacted with HCV, nor the heterologous bank vole hepacivirus. Co-occurrence of RNA and antibodies was found in 3 of 57 PCR-positive bank vole sera (5.3%). Our data enable new hypotheses regarding HCV evolution and encourage efforts to develop rodent surrogate models for HCV. [ABSTRACT FROM AUTHOR]
- Published
- 2013
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20. Evidence for widespread infection of African bats with Crimean-Congo hemorrhagic fever-like viruses.
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Müller, Marcel A., Devignot, Stéphanie, Lattwein, Erik, Corman, Victor Max, Maganga, Gaël D., Gloza-Rausch, Florian, Binger, Tabea, Vallo, Peter, Emmerich, Petra, Cottontail, Veronika M., Tschapka, Marco, Oppong, Samuel, Drexler, Jan Felix, Weber, Friedemann, Leroy, Eric M., and Drosten, Christian
- Published
- 2016
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21. Corrigendum: Bats host major mammalian paramyxoviruses.
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Drexler, Jan Felix, Corman, Victor Max, Müller, Marcel Alexander, Maganga, Gael Darren, Vallo, Peter, Binger, Tabea, Gloza-Rausch, Florian, Cottontail, Veronika M., Rasche, Andrea, Yordanov, Stoian, Seebens, Antje, Knörnschild, Mirjam, Oppong, Samuel, Sarkodie, Yaw Adu, Pongombo, Célestin, Lukashev, Alexander N., Schmidt-Chanasit, Jonas, Stöcker, Andreas, Carneiro, Aroldo José Borges, and Erbar, Stephanie
- Published
- 2014
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22. Highly Divergent Hepaciviruses from African Cattle.
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Corman, Victor Max, Grundhoff, Adam, Baechlein, Christine, Fischer, Nicole, Gmyl, Anatoly, Wollny, Robert, Dei, Dickson, Ritz, Daniel, Binger, Tabea, Adankwah, Ernest, Marfo, Kwadwo Sarfo, Annison, Lawrence, Annan, Augustina, Adu-Sarkodie, Yaw, Oppong, Samuel, Becher, Paul, Drosten, Christian, and Drexler, Jan Felix
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HEPATITIS C virus , *PHYLOGENY , *NUCLEOTIDE sequence , *CATTLE diseases , *VIRAL load - Abstract
The hepatitis C virus (HCV; genus Hepacivirus) is a highly relevant human pathogen. Unique hepaciviruses (HV) were discovered recently in animal hosts. The direct ancestor of HCV has not been found, but the genetically most closely related animal HVs exist in horses. To investigate whether other peridomestic animals also carry HVs, we analyzed sera from Ghanaian cattle for HVs by reverse transcription-PCR (RT-PCR). Nine of 106 specimens from different sampling sites contained HV RNA (8.5%) at median viral loads of 1.6 ×105 copies/ml. Infection seemed unrelated to cattle age and gender. Near-full-genome sequencing of five representative viruses confirmed taxonomic classifications. Cattle HVs formed two distinct phylogenetic lineages that differed by up to 17.7% on the nucleotide level in the polyprotein-encoding region, suggesting cocirculation of different virus subtypes. A conserved microRNA122-binding site in the 5′ internal ribosomal entry site suggested liver tropism of cattle HVs. Phylogenetic analyses suggested the circulation of HVs in cattle for several centuries. Cattle HVs were genetically highly divergent from all other HVs, including HCV. HVs from genetically related equine and bovine hosts were not monophyletic, corroborating host shifts during the evolution of the genus Hepacivirus. Similar to equine HVs, the genetic diversity of cattle HVs was low compared to that of HCV genotypes. This suggests an influence of the human-modified ecology of peridomestic animals on virus diversity. Further studies should investigate the occurrence of cattle HVs in other geographic areas and breeds, virus pathogenicity in cattle, and the potential exposure of human risk groups, such as farmers, butchers, and abattoir workers. [ABSTRACT FROM AUTHOR]
- Published
- 2015
- Full Text
- View/download PDF
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