Random PCR and ultracentrifugation increases sensitivity and throughput of VIDISCA for screening of pathogens in clinical specimens

Le Van Tan; H. Rogier van Doorn; Lia van der Hoek; Vo Minh Hien; Maarten F. Jebbink; Do Quang Ha; Jeremy Farrar; Nguyen Van Vinh Chau; Menno D. de Jong

doi:10.3855/jidc.1087

Random PCR and ultracentrifugation increases sensitivity and throughput of VIDISCA for screening of pathogens in clinical specimens

Authors

Le Van Tan Oxford University Clinical Research Unit, 190 Ben Ham Tu, District 5, Ho Chi Minh City, Vietanm
H. Rogier van Doorn Oxford University Clinical Research Unit, 190 Ben Ham Tu, District 5, Ho Chi Minh City, Vietanm; Centre for Tropical Medicine, Oxford University, U.K
Lia van der Hoek Department of Medical Microbiology, Academic Medical Center, University of Amsterdam, Amsterdam, The Netherlands
Vo Minh Hien Hospital for Tropical Diseases, Ho Chi Minh City, Vietnam
Maarten F. Jebbink Department of Medical Microbiology, Academic Medical Center, University of Amsterdam, Amsterdam, The Netherlands
Do Quang Ha Oxford University Clinical Research Unit, Hospital for Tropical Diseases, Ho Chi Minh City, Vietnam
Jeremy Farrar Oxford University Clinical Research Unit, Hospital for Tropical Diseases, Ho Chi Minh City, Vietnam; Centre for Tropical Medicine, Oxford University, U.K
Nguyen Van Vinh Chau Hospital for Tropical Diseases, Ho Chi Minh City, Vietnam
Menno D. de Jong Oxford University Clinical Research Unit, Hospital for Tropical Diseases, Ho Chi Minh City, Vietnam; Centre for Tropical Medicine, Oxford University, U.K; Department of Medical Microbiology, Academic Medical Center, University of Amsterdam, Amsterdam

DOI:

https://doi.org/10.3855/jidc.1087

Keywords:

random PCR, VIDISCA, ultracentrifugatiaon, virus discovery

Abstract

Introduction: Virus discovery based on cDNA-AFLP (VIDISCA) is a sequence-independent virus discovery method that was recently developed and successfully used to characterize unknown viruses in cell cultures. Its applicability, however, is limited by its low sensitivity.

Methodology: We evaluated whether the introduction of prior amplification of target sequences by random PCR (rPCR) increases the sensitivity of this method to improve its use on clinical specimens. In addition, ultracentrifugation was added to the protocol to allow for pooling of multiple samples, thereby increasing analytical throughput of the VIDSCA.

Results: We showed that rPCR enhanced the sensitivity of VIDISCA by 100-fold for two out of four viruses in different clinical samples, and that the ultracentrifugation step allowed for analyzing samples of large volumes (4 ml) and simultaneous processing of multiple (~40) clinical specimens.

Conclusions: We conclude that this modified VIDISCA protocol is a relatively easy method to use for screening of large numbers of clinical samples that are suspected to contain previously unrecognized pathogens, in settings where ultradeep sequencing platforms are not available.

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Published

2010-07-19

How to Cite

Tan LV, van Doorn HR, van der Hoek L, Minh Hien V, F. Jebbink M, Quang Ha D, Farrar J, Van Vinh Chau N, D. de Jong M (2010) Random PCR and ultracentrifugation increases sensitivity and throughput of VIDISCA for screening of pathogens in clinical specimens. J Infect Dev Ctries 5:142–148. doi: 10.3855/jidc.1087

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Issue

Vol. 5 No. 02: February 2011

Section

Technical Notes

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