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Original Articles
Development of Molecular Diagnosis Using Multiplex Real-Time PCR and T4 Phage Internal Control to Simultaneously Detect Cryptosporidium parvum, Giardia lamblia, and Cyclospora cayetanensis from Human Stool Samples
Ji-Hun Shin, Sang-Eun Lee, Tong Soo Kim, Da-Won Ma, Shin-Hyeong Cho, Jong-Yil Chai, Eun-Hee Shin
Korean J Parasitol 2018;56(5):419-427.
Published online October 31, 2018
DOI: https://doi.org/10.3347/kjp.2018.56.5.419
This study aimed to develop a new multiplex real-time PCR detection method for 3 species of waterborne protozoan parasites (Cryptosporidium parvum, Giardia lamblia, and Cyclospora cayetanensis) identified as major causes of traveler’s diarrhea. Three target genes were specifically and simultaneously detected by the TaqMan probe method for multiple parasitic infection cases, including Cryptosporidium oocyst wall protein for C. parvum, glutamate dehydrogenase for G. lamblia, and internal transcribed spacer 1 for C. cayetanensis. Gene product 21 for bacteriophage T4 was used as an internal control DNA target for monitoring human stool DNA amplification. TaqMan probes were prepared using 4 fluorescent dyes, FAMTM, HEXTM, Cy5TM, and CAL Fluor Red® 610 on C. parvum, G. lamblia, C. cayetanensis, and bacteriophage T4, respectively. We developed a novel primer-probe set for each parasite, a primer-probe cocktail (a mixture of primers and probes for the parasites and the internal control) for multiplex real-time PCR analysis, and a protocol for this detection method. Multiplex real-time PCR with the primer-probe cocktail successfully and specifically detected the target genes of C. parvum, G. lamblia, and C. cayetanensis in the mixed spiked human stool sample. The limit of detection for our assay was 2×10 copies for C. parvum and for C. cayetanensis, while it was 2×103 copies for G. lamblia. We propose that the multiplex real-time PCR detection method developed here is a useful method for simultaneously diagnosing the most common causative protozoa in traveler’s diarrhea.

Citations

Citations to this article as recorded by  Crossref logo
  • A rapid and ultrasensitive CRISPR/Cas12a-based assay for the accurate identification of T-even type phages
    Chenhang Jiang, Yang Li, Ping Yu, Mengjun Fang, Di Huang, Xiangming Fang, Zhinan Xu
    Biotechnology Letters.2025;[Epub]     CrossRef
  • Assessment of Cryptosporidium spp. Sub-Families and Giardia duodenalis Assemblages A and B in Ghanaian HIV Patients, Including Socio-Economic, Clinical, and Immunological Associations
    Lynn Glyschewski, Hagen Frickmann, Fred Stephen Sarfo, Betty Roberta Norman, Albert Dompreh, Emmanuel Acheamfour-Akowuah, Martin Kofi Agyei, Shadrack Osei Asibey, Richard Boateng, Edmund Osei Kuffour, Veronica Di Cristanziano, Sven Poppert, Felix Weinreic
    Infectious Disease Reports.2025; 17(5): 129.     CrossRef
  • Evaluation of molecular-based methods for the detection and quantification of Cryptosporidium spp. in wastewater
    Oumaima Hachimi, Rebecca Falender, Gabriel Davis, Rispa Vranka Wafula, Melissa Sutton, June Bancroft, Paul Cieslak, Christine Kelly, Devrim Kaya, Tyler Radniecki
    Science of The Total Environment.2024; 947: 174219.     CrossRef
  • Development of duplex real‐time PCR for quick detection of cryptosporidiosis in goats
    Atul Kumar Sharma, K. Gururaj, Rama Sharma, Anjana Goel, Souvik Paul, Dinesh Kumar Sharma
    Cell Biochemistry and Function.2023; 41(1): 45.     CrossRef
  • The Importance of Endoscopy with Biopsy: Real-World Evidence of Gastrointestinal Involvement in Primary Immunodeficiency in Two Main Northern Italian Centres
    Stefania Nicola, Francesco Cinetto, Stefano Della Mura, Luca Lo Sardo, Elena Saracco, Ilaria Vitali, Riccardo Scarpa, Helena Buso, Vera Bonato, Claudia Discardi, Giovanni Rolla, Carla Felice, Marcello Rattazzi, Luisa Brussino
    Biomedicines.2023; 11(1): 170.     CrossRef
  • Efficacy of a membrane concentration method combined with real-time PCR for detection of Giardia and Cryptosporidium in drinking water
    Jiang Jingyi, Yao Ping, Xu Jian, Chen Jia, Mao Xujian, Li Qiong, Tu Bowen, Wang Fengming
    Letters in Applied Microbiology.2023;[Epub]     CrossRef
  • Bacteriophages: from Isolation to Application
    Abdallah Abdelsattar, Alyaa Dawoud, Salsabil Makky , Rana Nofal, Ramy Aziz, Ayman El-Shibiny
    Current Pharmaceutical Biotechnology.2022; 23(3): 337.     CrossRef
  • Comparative Evaluation of Real-Time Screening PCR Assays for Giardia duodenalis and of Assays Discriminating the Assemblages A and B
    Felix Weinreich, Andreas Hahn, Kirsten Alexandra Eberhardt, Simone Kann, Torsten Feldt, Fred Stephen Sarfo, Veronica Di Cristanziano, Hagen Frickmann, Ulrike Loderstädt
    Microorganisms.2022; 10(7): 1310.     CrossRef
  • Review on Cyclosporiasis Outbreaks and Potential Molecular Markers for Tracing Back Investigations
    Junqiang Li, Feifei Xu, Md Robiul Karim, Longxian Zhang
    Foodborne Pathogens and Disease.2022; 19(12): 796.     CrossRef
  • Multiplex Molecular Point-of-Care Test for Syndromic Infectious Diseases
    Hanbi Kim, Hee Jae Huh, Eunkyoung Park, Doo-Ryeon Chung, Minhee Kang
    BioChip Journal.2021; 15(1): 14.     CrossRef
  • Comparative Performance of Eight PCR Methods to Detect Cryptosporidium Species
    Damien Costa, Louise Soulieux, Romy Razakandrainibe, Louise Basmaciyan, Gilles Gargala, Stéphane Valot, Frédéric Dalle, Loic Favennec
    Pathogens.2021; 10(6): 647.     CrossRef
  • A review on application of next-generation sequencing methods for profiling of protozoan parasites in water: Current methodologies, challenges, and perspectives
    N.P. Mthethwa, I.D. Amoah, P. Reddy, F. Bux, S. Kumari
    Journal of Microbiological Methods.2021; 187: 106269.     CrossRef
  • Comparison of Three Real-Time PCR Assays Targeting the SSU rRNA Gene, the COWP Gene and the DnaJ-Like Protein Gene for the Diagnosis of Cryptosporidium spp. in Stool Samples
    Felix Weinreich, Andreas Hahn, Kirsten Alexandra Eberhardt, Torsten Feldt, Fred Stephen Sarfo, Veronica Di Cristanziano, Hagen Frickmann, Ulrike Loderstädt
    Pathogens.2021; 10(9): 1131.     CrossRef
  • Advances in Cyclosporiasis Diagnosis and Therapeutic Intervention
    Junqiang Li, Zhaohui Cui, Meng Qi, Longxian Zhang
    Frontiers in Cellular and Infection Microbiology.2020;[Epub]     CrossRef
  • Comparison of commercial and in-house real-time PCR platforms for 15 parasites and microsporidia in human stool samples without a gold standard
    Thomas Köller, Andreas Hahn, Enkhtsetseg Altangerel, Jaco J. Verweij, Olfert Landt, Simone Kann, Denise Dekker, Jürgen May, Ulrike Loderstädt, Andreas Podbielski, Hagen Frickmann
    Acta Tropica.2020; 207: 105516.     CrossRef
  • Biochemical Markers of the Functional State of the Liver during Giardiasis
    D. V. Morozenko, K. V. Gliebova, S. V. Ivannikova, O. G. Geyderikh, O. V. Shapovalova, A. V. Derevyanko
    Ukraïnsʹkij žurnal medicini, bìologìï ta sportu.2019; 4(2): 149.     CrossRef
  • Molecular epidemiology of Giardia and Cryptosporidium infections – What's new?
    R.C.A. Thompson, A. Ash
    Infection, Genetics and Evolution.2019; 75: 103951.     CrossRef
  • Cyclospora cayetanensis and Cyclosporiasis: An Update
    Sonia Almeria, Hediye N. Cinar, Jitender P. Dubey
    Microorganisms.2019; 7(9): 317.     CrossRef
  • 10,696 View
  • 294 Download
  • 19 Web of Science
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Internal Amplification Control for a Cryptosporidium Diagnostic PCR: Construction and Clinical Evaluation
Yousry Hawash, M. M. Ghonaim, Ayman S. Al-Hazmi
Korean J Parasitol 2015;53(2):147-154.
Published online April 22, 2015
DOI: https://doi.org/10.3347/kjp.2015.53.2.147
Various constituents in clinical specimens, particularly feces, can inhibit the PCR assay and lead to false-negative results. To ensure that negative results of a diagnostic PCR assay are true, it should be properly monitored by an inhibition control. In this study, a cloning vector harboring a modified target DNA sequence (?375 bp) was constructed to be used as a competitive internal amplification control (IAC) for a conventional PCR assay that detects ?550 bp of the Cryptosporidium oocyst wall protein (COWP) gene sequence in human feces. Modification of the native PCR target was carried out using a new approach comprising inverse PCR and restriction digestion techniques. IAC was included in the assay, with the estimated optimum concentration of 1 fg per reaction, as duplex PCR. When applied on fecal samples spiked with variable oocysts counts, ?2 oocysts were theoretically enough for detection. When applied on 25 Cryptosporidium-positive fecal samples of various infection intensities, both targets were clearly detected with minimal competition noticed in 2-3 samples. Importantly, both the analytical and the diagnostic sensitivities of the PCR assay were not altered with integration of IAC into the reactions. When tried on 180 randomly collected fecal samples, 159 were Cryptosporidium-negatives. Although the native target DNA was absent, the IAC amplicon was obviously detected on gel of all the Cryptosporidium-negative samples. These results imply that running of the diagnostic PCR, inspired with the previously developed DNA extraction protocol and the constructed IAC, represents a useful tool for Cryptosporidium detection in human feces.

Citations

Citations to this article as recorded by  Crossref logo
  • Critical evaluation of current isolation, detection, and genotyping methods of Cryptosporidium species and future direction
    Rabbee G. Mahmudunnabi, Surasak Kasetsirikul, Narshone Soda, Mohamed Sallam, Amandeep Singh Pannu, Nam-Trung Nguyen, Helen Stratton, Muhammad J. A. Shiddiky
    Environmental Science: Water Research & Technology.2024; 10(7): 1527.     CrossRef
  • Nucleic acid extraction without electrical equipment via magnetic nanoparticles in Pasteur pipettes for pathogen detection
    Jia Kang, Yang Li, Yan Zhao, Yanling Wang, Cuiping Ma, Chao Shi
    Analytical Biochemistry.2021; 635: 114445.     CrossRef
  • Comparative evaluation of Cryptosporidium infection in malnourished and well-nourished children: Parasitic infections are affected by the interaction of nutritional status and socio-demographic characteristics
    Solmaz Madadi, Mahmoud Mahami-Oskouei, Mandana Rafeey, Adel Spotin, Nayyereh Aminisani, Leyla Mahami-Oskouei, Roghayeh Ghoyounchi, Reza Berahmat
    Comparative Immunology, Microbiology and Infectious Diseases.2020; 68: 101406.     CrossRef
  • An optimized assay for detecting Encephalitozoon intestinalis and Enterocytozoon bieneusi in dairy calf feces using polymerase chain reaction technology
    M. C. Jenkins, C. N. O’Brien, C. Parker
    Journal of Parasitic Diseases.2019; 43(1): 75.     CrossRef
  • Coproscopy and molecular screening for detection of intestinal protozoa
    Marawan Abu-Madi, Sonia Boughattas, Jerzy M. Behnke, Aarti Sharma, Ahmed Ismail
    Parasites & Vectors.2017;[Epub]     CrossRef
  • Development of Internal PCR Control (IPC) for Human Mitochondrial DNA Typing Kit
    Ishar Seri Miria, Abdullah Nur Azeela, Zainuddin Zafarina
    Journal of Biological Sciences.2017; 17(8): 410.     CrossRef
  • RT-PCR specific for Cryspovirus is a highly sensitive method for detecting Cryptosporidium parvum oocysts
    Mark Jenkins, Celia O'Brien, Raymond Fetterer, Monica Santin
    Food and Waterborne Parasitology.2016; 5: 14.     CrossRef
  • An Improved PCR-RFLP Assay for Detection and Genotyping of Asymptomatic Giardia lamblia Infection in a Resource-Poor Setting
    Yoursry Hawash, M. M. Ghonaim, S. S. Al-Shehri
    The Korean Journal of Parasitology.2016; 54(1): 1.     CrossRef
  • Clinical consequences of polymerase chain reaction‐based diagnosis of intestinal parasitic infections
    Lucas H Rijsman, Jan F Monkelbaan, Johannes G Kusters
    Journal of Gastroenterology and Hepatology.2016; 31(11): 1808.     CrossRef
  • 13,322 View
  • 129 Download
  • 7 Web of Science
  • Crossref