Development of bioassay for pathogenecity testing of Ureaplasma urealyticum as part of host-pathogen communication
Abstract: Bioassay of
Ureaplasma urealyticum is necessary for detection as well as determination of
pathogenic factors in order to understand the pathogenesis of diseases
associate with ureaplasma infection. Cultivation and verification of ureaplasma
is the first step of this study in the purpose of discovering sensitive method
for ureaplasma detection. Cultivation of ureaplasma either in liquid or in
solid media are able to detect the existence of ureaplasma in samples analyzed.
However, application of PCR using specific primers to be compatible with urease
gene (ure) would confirm the presence of ureaplasma. The pathogenicity of
ureaplasma is potentially monitored using reporter gene as a marker for gene
expression. IceC was chosen as reporter gene for ureaplasma pathogenic
determination as the gene has great sensitivity, easily detectable and
quantitated in simple method of ice nucleation assay. Transposon 916 (Tn916)
was selected as a vector for iceC gene to transform ureaplasma. The application
of recombinant Tn916-iceC which is considered as pUI, allow detection of
ureaplasma activities when transform ureaplasma is tested by ice nucleation
assay. It was expected that ureaplasma transformation is the manifestation of
mutagenesis which interfere genes responsible for bacterial pathogenicity, in
order pathogenesis of bacterial infection to be analyzed accurately. IgA1
protease is considered to be an important factor for ureaplasma pathogenicity
as the enzyme is required for successful colonization. Identification of iga
gene and determination of IgA1 protease
activity are important for understanding the pathogenesis of ureaplasma
infection. Putative iga gene of Mycoplasma genitalium was used as a reference
to identify the presence of iga nucleotide sequence in U. urealyticum.
Convincing evidence were obtained after PCR amplification of ureaplasma DNA
using primers designed to be compatible with putative iga gene of M. genitalium
followed by the discovery of 100% sequence homology of amplified ureaplasma iga gene and iga gene of M.
genitalium mentioned in establish data. IgA1 protease activity of U. urealytium
has been detectable in the cell rather than in media culture, suggesting that IgA1 protease is not secreted
out of cell. It was proofed that IgA1 protease is membrane bound enzyme capable
of digesting IgA1 in mucosal tissues of various organs and considered as
potential virulence factor for ureaplasma that cause disease or gain entry to
mucosal membrane. The existence of IgA1 protease activity in bacterial plasma membrane
would have implication in ureaplasma management such as diagnosis and therapy
of ureaplasma infection.
Keywords: Ureaplasma
detection, Ureaplasma pathogenicity, IceC reporter gene, IgA1 protease, M.
genitalium putative gene
Author: Purnomo Soeharso
Journal Code: jpkedokterangg050137

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