TY - JOUR
T1 - ECC-RT-PCR
T2 - A new method to determine the viability and infectivity of Giardia cysts
AU - Alum, Absar
AU - Sbai, Basel
AU - Asaad, Hamas
AU - Rubino, Joseph R.
AU - Khalid Ijaz, M.
N1 - Funding Information:
Dr Alum's research is supported by Reckitt Benckiser, and JRR and MKI are engaged in R&D work at Reckitt Benckiser Inc., Montvale, NJ, USA.
PY - 2012/5
Y1 - 2012/5
N2 - Background: Giardia sp is a major cause of diarrheal illness worldwide, and millions of people are infected each year. Rapid methods to determine the infectivity and virulence of isolates are critical for the development of intervention strategies to control the transmission of Giardia sp cysts, which occurs through contaminated surfaces, food, and water. However, determining the viability, infectivity, and virulence of Giardia sp cysts using molecular methods is a technical challenge because of the lack of a cell culture model. Method: This study was designed to evaluate mRNA expression in trophozoites and to assess trophozoite attachment to cell monolayer and changes in transcellular resistance as an indicator of Giardia sp viability and infectivity. Heat shock mRNA in Giardia cysts and variant-specific protein (VSP) mRNA in trophozoites were quantified by reverse transcription polymerase chain reaction (RT-PCR). C2bb (Caco-2) cells were grown on transwell chambers to study the attachment of trophozoites, changes in transcellular resistance, and expression of VSP in trophozoites. Results: The results of these molecular and cell culture studies indicate a direct linear correlation between the viability and infectivity of fresh stocks of Giardia sp cysts. The attachment of trophozoites to cell monolayer, expression of VSP, and change in the transcellular resistance was directly correlated with their infectivity in neonatal mice. PCR was successfully combined with the electrophysiological analysis of cell culture (ECC-RT-PCR) post-trophozoite attachment. Conclusion: This study shows that the ECC-RT-PCR, a new integrated cell culture assay, can be used as a rapid and cost-effective tool for assessing the viability and infectivity of environmental isolates of Giardia sp cysts.
AB - Background: Giardia sp is a major cause of diarrheal illness worldwide, and millions of people are infected each year. Rapid methods to determine the infectivity and virulence of isolates are critical for the development of intervention strategies to control the transmission of Giardia sp cysts, which occurs through contaminated surfaces, food, and water. However, determining the viability, infectivity, and virulence of Giardia sp cysts using molecular methods is a technical challenge because of the lack of a cell culture model. Method: This study was designed to evaluate mRNA expression in trophozoites and to assess trophozoite attachment to cell monolayer and changes in transcellular resistance as an indicator of Giardia sp viability and infectivity. Heat shock mRNA in Giardia cysts and variant-specific protein (VSP) mRNA in trophozoites were quantified by reverse transcription polymerase chain reaction (RT-PCR). C2bb (Caco-2) cells were grown on transwell chambers to study the attachment of trophozoites, changes in transcellular resistance, and expression of VSP in trophozoites. Results: The results of these molecular and cell culture studies indicate a direct linear correlation between the viability and infectivity of fresh stocks of Giardia sp cysts. The attachment of trophozoites to cell monolayer, expression of VSP, and change in the transcellular resistance was directly correlated with their infectivity in neonatal mice. PCR was successfully combined with the electrophysiological analysis of cell culture (ECC-RT-PCR) post-trophozoite attachment. Conclusion: This study shows that the ECC-RT-PCR, a new integrated cell culture assay, can be used as a rapid and cost-effective tool for assessing the viability and infectivity of environmental isolates of Giardia sp cysts.
KW - Giardiasis
KW - Infectious Giardia cysts
KW - Molecular diagnostic method
UR - http://www.scopus.com/inward/record.url?scp=84859629395&partnerID=8YFLogxK
UR - http://www.scopus.com/inward/citedby.url?scp=84859629395&partnerID=8YFLogxK
U2 - 10.1016/j.ijid.2012.01.004
DO - 10.1016/j.ijid.2012.01.004
M3 - Article
C2 - 22390842
AN - SCOPUS:84859629395
SN - 1201-9712
VL - 16
SP - e350-e353
JO - International Journal of Infectious Diseases
JF - International Journal of Infectious Diseases
IS - 5
ER -