A. El Hussein scite author profile

A. El Hussein

3Publications

49Citation Statements Received

45Citation Statements Given

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Affiliations

Ministry of Science ICT and Future Planning, Colorado State University

Publications

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Asynchronous Mixed Infection of Culicoides variipennis with Bluetongue Virus Serotypes 10 and 17

Hussein

Ramig

Holbrook³

et al. 1989

Journal of General Virology

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SUMMARYCulicoides variipennis (Diptera: Ceratopogonidae) the primary vector of bluetongue virus (BTV) in the U.S.A. were asynchronously mixedly infected with two BTV serotypes (BTV-10 and BTV-17); flies first ingested a blood meal that contained BTV-17 and 1, 3, 5, 7, and 9 days later selected flies ingested a second blood meal that contained BTV-10. Control flies ingested each parental virus separately, or both viruses simultaneously, in a single blood meal. Electrophoretic analysis of progeny virus clones indicated that superinfection with BTV-10 occurred when the flies ingested the second virus 1, 3 and 5 days post-initial infection. Parental BTV-17 and reassortant virus clones were isolated from these flies, but parental BTV-10 virus was not isolated from any flies. Reassortant clone frequencies were 67~, 71% and 17% when superinfection occurred on days 1, 3 and 5 after initial infection, respectively, as compared to 48 ~ for simultaneously infected flies. Only parental BTV-17 clones were isolated from flies that ingested the second virus on days 7 and 9 after initial BTV-17 infection. The results indicated that interference to superinfection occurred in C. variipennis by 5 days and flies were refractory to superinfection by 7 days post-initial infection.

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Primary investigation of 31 infants with suspected congenital rubella syndrome in Sudan

Adam

Hussein

Eragi³

2010

Clinical Microbiology and Infection

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Between 2005 and 2006, clinical specimens were collected from 31 infants with suspected congenital rubella syndrome (CRS) who presented at six hospitals in Khartoum, Sudan. Eleven (35.5%) were laboratory confirmed as CRS cases by testing for anti-rubella IgM, IgG and viral genome. For the first time in Sudan, the rubella virus genome was directly detected in clinical specimens of six CRS cases and two viruses were isolated in cell culture. Phylogenetic analysis suggested that three genotypes of rubella virus (RV; 1E, 2B and 1G) were co-circulating in Sudan. The study introduced the methodology for CRS confirmation and surveillance in Sudan and provides preliminary data.

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Detection of bluetongue virus antigens in Culicoides variipennis by enzyme immunoassay

et al. 1989

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A solid-phase enzyme immunoassay (EIA) was developed to detect bluetongue (BT) virus antigens in infected cell cultures and in suspensions of infected Culicoides variipennis midges. The technique was equally sensitive for detecting the five U.S. BT virus serotypes (2, 10, 11, 13, and 17) in cell cultures. EIA reliably detected about 3.8 loglo median tissue culture infective doses per ml of BT virus in infected cell culture lysates. The EIA readily detected virus antigens in pools of midges infected with BT serotypes 2, 10, 11, 13, and 17 and contained 2.3 to 4.8 loglo median tissue culture infective doses per ml of BT virus. The technique was sensitive enough to detect a single infected midge in a pool with 99 noninfected midges. The EIA may be a sensitive and rapid alternative to virus isolation for surveillance of BT viruses in vector populations.

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A. El Hussein

Asynchronous Mixed Infection of Culicoides variipennis with Bluetongue Virus Serotypes 10 and 17

Primary investigation of 31 infants with suspected congenital rubella syndrome in Sudan

Detection of bluetongue virus antigens in Culicoides variipennis by enzyme immunoassay

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