Article citationsMore>>
Wagner, K.S., White, J.M., Neal, S., Crowcroft, N.S., Kupreviciene, N., Paberza, R., Lucenko, I., Joks, U., Akbas, E., Alexandrou-Athanassoulis, H., Detcheva, A., Vuopio, J., von Hunolstein, C., Murphy, P.G., Andrews, N., Members of the Diphtheria Surveillance Network (DIPNET) and Efstratiou, A. (2011) Screening for Corynebacterium diphtheriae and Corynebacterium ulcerans in patients with upper respiratory tract infections 2007-2008: A multicentre European study. Clinical Microbiology and Infection, 17, 519-525.
doi:10.1111/j.1469-0691.2010.03269.x
has been cited by the following article:
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TITLE:
Plasmid instability when the hsp60 gene promoter is used to express the protective non-toxic fragment B of the diphtheria toxin in recombinant BCG
AUTHORS:
Dilzamar V. Nascimento, Odir A. Dellagostin, Raphael Hirata Junior, Geraldo M. B. Pereira, Ana Luiza Mattos-Guaraldi, Geraldo R. Garcia Armôa
KEYWORDS:
BCG Vaccine; Recombinant BCG; Fragment B of Diphtheria Toxin; Anti-Diphtheria Vaccine
JOURNAL NAME:
American Journal of Molecular Biology,
Vol.3 No.2,
April
30,
2013
ABSTRACT:
The genetic modification of the live attenuated Mycobacterium
bovis BCG to deliver a protective Corynebacterium diphtheriae antigen in vivo could be a safer and less costly
alternative to the new and more expensive DTP vaccines available today, in
particular to third world-countries. The stability of expression of
heterologous antigens in BCG, however, is a major challenge to the use of live
recombinant bacteria in vaccine development and appears to be dependent to a
certain extent, on a genetic compatibility between the expression cassette
within the plasmid construct and the mycobacterium host. In the quest for the
best recombinant BCG transformant to express the dtb gene of C. diphtheriae we generated two new rBCG strains by transforming the Moreau substrain of BCG with the mycobacterial expression vectors pUS973
and pUS977, each one carrying a different promoter to drive the expression of
the target antigen. After transformation recombinant BCG clones were selected
on Middlebrook 7H10 kanamycin Agar plates, expanded in Middlebrook 7H9
kanamycin Broth and analyzed by agarose gel electrophoresis and immunoblotting.
rBCGs transformed with the construct carrying the weak PAN promoter from M. paratuberculosis stably expressed the dtb gene. Conversely, rBCGs transformed
with the construct carrying the strong mycobacterium hsp60 promoter were unstable and consequently unfit for the expression
of the C. diphtheriae gene.
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