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1.
Article in English | IMSEAR | ID: sea-133954

ABSTRACT

 Fifty clinical isolates of Burkholderia(Pseudomonal) pseudomallei were tested by broth microdilution technique for susceptibility to OPC-17116 , a new 5-methyl substituted quinolone. The minimul inhibitory concentration (MIC) range was 1-8 µg/ml. The MIC 50 and MIC 90 were 2.6 µg/ml and 0.4 µg/ml, respectively.

2.
Article in English | IMSEAR | ID: sea-133915

ABSTRACT

\ CD4 lymphocyte (T helper cell) plays a major role in the regulation of the immune response.\  Decrease in number of CD4 lymphocyte, due to being infected and destroyed by human immunodeficiency virus (Hiv), is the key index for monitoring the stage of disease progression.\  The appropriate treatment thus can be given to the patients at the right time corresponding to the need of the patients.\  By direct immunofluorescence technique using monoclonal antibodies, CD4, CD8 lymphocyte and CD4/CD8 ratio were enumerated and calculated.\  In 37 normal healthy controls (male 20, female 17), aged 26  5 years, the percentage of CD4 and CD8 lymphocytes were 38  8 (range : 23-60) and 28  7 (17-42), the absolute number of CD4 and CD8 lymphocytes were 956  277 cell/mm3 (545 \– 1504 cell/mm3 ) and 701  252 (348-1416) respectively.\  The CD4/CD8 ratio was 1.42  0.34 (0.72-2.48)\ We have studied 61 HIV-infected cases by categorizing them into asymtomatic HIV infection, AIDS relaed complex (ARC), and the full-blown AIDS.\  The results were tabulated in table 2.\  The best prognostic index was the absolute number of CD4 lymphocyte which could also differentiate among the various stages of HIV-infected patients; asymptomatic HIV infection (623  347; range : 92-1350), AIDS related complex (ARC) (347  365; 35-1509) and the full blown AIDS (137  130; 9-472).Key words : CD4 lymphocyte, CD4/CD8 ratio, AIDS, Immunofluorescence

3.
Article in English | IMSEAR | ID: sea-133891

ABSTRACT

 Melioidosis is still a fatal disease with high mortality rate, especially, in septicemic melioidosis.  Clinical manifestations of this disease are protean and mimick those of other infectious diseases.  Laboratory diagnosis is often too late as the patients died before the hemocultures were positive.  Thus, measurement of antibody level is of the most appropriate diagnostic approach.  In the past, the use of crude or non-specific antigens may account for false-positive results and high antibody levels in normal people in endemic areas.  In this study, a search for specific antigens of P. pseudomallei was carried out by using SDS-Page and immunoblot techniques.  The sonic extracted antigens obtained from 30 isolates of P. pseudomallei were analysed.  They all showed the same protein profiles.  The sonicated antigens which were found to be specific for P. pseudomallei had the melecular weight of 21, 18, 15.5 and 13 kDa. 

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