An international external quality assessment of nucleic acid amplification of herpes simplex virus

Lottie Schloss; Anton M van Loon; Paola Cinque; Graham Cleator; José-Manuel Echevarria; Kerstin I Falk; Paul Klapper; Jurjen Schirm; Bent Faber Vestergaard; Hubert Niesters; Therese Popow-Kraupp; Wim Quint; Annika Linde

doi:10.1016/S1386-6532(03)00003-9

An international external quality assessment of nucleic acid amplification of herpes simplex virus

Lottie Schloss, Anton M van Loon, Paola Cinque, Graham Cleator, José-Manuel Echevarria, Kerstin I Falk, Paul Klapper, Jurjen Schirm, Bent Faber Vestergaard, Hubert Niesters, Therese Popow-Kraupp, Wim Quint, Annika Linde

Research output: Contribution to journal › Article › Academic › peer-review

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Abstract

BACKGROUND: There is an increasing awareness of the need for external quality control of diagnostic virology.

OBJECTIVES: To assess the quality of nucleic acid amplification tests (NAT) of herpes simplex within Europe.

STUDY DESIGN: Herpes simplex virus (HSV) proficiency panels were produced at the Swedish Institute for Infectious Disease Control on behalf of the European Union Concerted Action for Quality Control of Nucleic Acid Amplification in 1999 and 2000. Nine reference laboratories evaluated the production process. Each panel consisted of 12 coded samples with various concentrations of inactivated, freeze-dried HSV type 1 (HSV-1), and HSV type 2 (HSV-2), or negative controls. Positive samples included HSV-1 and HSV-2 in a range of concentrations (2 x 10(2) to 2 x 10(7) genome copies per ml) similar to those found in cerebrospinal fluids from patients with HSV encephalitis.

RESULTS: Sixty-six participants reported a total of 76 data sets for panel 1, and 71 reported 78 data sets for panel 2. The majority of the participants employed qualitative 'in-house' polymerase chain reaction (PCR) methods, either in a single, nested or semi-nested format. For panel 2, 9 laboratories reported use of 'real-time' PCR in contrast to 3 for panel 1. Three laboratories submitted quantitative results on both panels. Thirty percent of the data sets had correct results for the entire panel 1. In 6 data sets (8%) a total of 11 false positive results were reported. For panel 2, 28% of the data sets had correct result. Nineteen false positive results were reported in 14 data sets (18%), but most of the incorrect results reflected a lack of test sensitivity.

CONCLUSIONS: The relatively high frequency of false positive results and the large number of false-negative results, albeit at low copy number, stress the need for improvement in the quality of HSV NAT and for external quality control programmes.

Original language	English
Pages (from-to)	175-785
Number of pages	11
Journal	Journal of Clinical Virology
Volume	28
Issue number	2
DOIs	https://doi.org/10.1016/S1386-6532(03)00003-9
Publication status	Published - Oct-2003
Externally published	Yes

Keywords

False Negative Reactions
False Positive Reactions
Herpes Simplex
Humans
International Cooperation
Laboratories
Polymerase Chain Reaction
Quality Assurance, Health Care
Quality Control
RNA, Viral
Reference Standards
Reproducibility of Results
Sensitivity and Specificity
Simplexvirus

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An international external quality assessment of nucleic acid amplification of herpes simplex virus
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Schloss, L., van Loon, A. M., Cinque, P., Cleator, G., Echevarria, J.-M., Falk, K. I., Klapper, P., Schirm, J., Vestergaard, B. F., Niesters, H., Popow-Kraupp, T., Quint, W., & Linde, A. (2003). An international external quality assessment of nucleic acid amplification of herpes simplex virus. Journal of Clinical Virology, 28(2), 175-785. https://doi.org/10.1016/S1386-6532(03)00003-9

@article{337c64fb09884c668c7f59bfca5578e6,

title = "An international external quality assessment of nucleic acid amplification of herpes simplex virus",

abstract = "BACKGROUND: There is an increasing awareness of the need for external quality control of diagnostic virology.OBJECTIVES: To assess the quality of nucleic acid amplification tests (NAT) of herpes simplex within Europe.STUDY DESIGN: Herpes simplex virus (HSV) proficiency panels were produced at the Swedish Institute for Infectious Disease Control on behalf of the European Union Concerted Action for Quality Control of Nucleic Acid Amplification in 1999 and 2000. Nine reference laboratories evaluated the production process. Each panel consisted of 12 coded samples with various concentrations of inactivated, freeze-dried HSV type 1 (HSV-1), and HSV type 2 (HSV-2), or negative controls. Positive samples included HSV-1 and HSV-2 in a range of concentrations (2 x 10(2) to 2 x 10(7) genome copies per ml) similar to those found in cerebrospinal fluids from patients with HSV encephalitis.RESULTS: Sixty-six participants reported a total of 76 data sets for panel 1, and 71 reported 78 data sets for panel 2. The majority of the participants employed qualitative 'in-house' polymerase chain reaction (PCR) methods, either in a single, nested or semi-nested format. For panel 2, 9 laboratories reported use of 'real-time' PCR in contrast to 3 for panel 1. Three laboratories submitted quantitative results on both panels. Thirty percent of the data sets had correct results for the entire panel 1. In 6 data sets (8%) a total of 11 false positive results were reported. For panel 2, 28% of the data sets had correct result. Nineteen false positive results were reported in 14 data sets (18%), but most of the incorrect results reflected a lack of test sensitivity.CONCLUSIONS: The relatively high frequency of false positive results and the large number of false-negative results, albeit at low copy number, stress the need for improvement in the quality of HSV NAT and for external quality control programmes.",

keywords = "False Negative Reactions, False Positive Reactions, Herpes Simplex, Humans, International Cooperation, Laboratories, Polymerase Chain Reaction, Quality Assurance, Health Care, Quality Control, RNA, Viral, Reference Standards, Reproducibility of Results, Sensitivity and Specificity, Simplexvirus",

author = "Lottie Schloss and {van Loon}, {Anton M} and Paola Cinque and Graham Cleator and Jos{\'e}-Manuel Echevarria and Falk, {Kerstin I} and Paul Klapper and Jurjen Schirm and Vestergaard, {Bent Faber} and Hubert Niesters and Therese Popow-Kraupp and Wim Quint and Annika Linde",

year = "2003",

month = oct,

doi = "10.1016/S1386-6532(03)00003-9",

language = "English",

volume = "28",

pages = "175--785",

journal = "Journal of Clinical Virology",

issn = "1386-6532",

publisher = "ELSEVIER SCIENCE BV",

number = "2",

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Schloss, L, van Loon, AM, Cinque, P, Cleator, G, Echevarria, J-M, Falk, KI, Klapper, P, Schirm, J, Vestergaard, BF, Niesters, H, Popow-Kraupp, T, Quint, W & Linde, A 2003, 'An international external quality assessment of nucleic acid amplification of herpes simplex virus', Journal of Clinical Virology, vol. 28, no. 2, pp. 175-785. https://doi.org/10.1016/S1386-6532(03)00003-9

TY - JOUR

T1 - An international external quality assessment of nucleic acid amplification of herpes simplex virus

AU - Schloss, Lottie

AU - van Loon, Anton M

AU - Cinque, Paola

AU - Cleator, Graham

AU - Echevarria, José-Manuel

AU - Falk, Kerstin I

AU - Klapper, Paul

AU - Schirm, Jurjen

AU - Vestergaard, Bent Faber

AU - Niesters, Hubert

AU - Popow-Kraupp, Therese

AU - Quint, Wim

AU - Linde, Annika

PY - 2003/10

Y1 - 2003/10

N2 - BACKGROUND: There is an increasing awareness of the need for external quality control of diagnostic virology.OBJECTIVES: To assess the quality of nucleic acid amplification tests (NAT) of herpes simplex within Europe.STUDY DESIGN: Herpes simplex virus (HSV) proficiency panels were produced at the Swedish Institute for Infectious Disease Control on behalf of the European Union Concerted Action for Quality Control of Nucleic Acid Amplification in 1999 and 2000. Nine reference laboratories evaluated the production process. Each panel consisted of 12 coded samples with various concentrations of inactivated, freeze-dried HSV type 1 (HSV-1), and HSV type 2 (HSV-2), or negative controls. Positive samples included HSV-1 and HSV-2 in a range of concentrations (2 x 10(2) to 2 x 10(7) genome copies per ml) similar to those found in cerebrospinal fluids from patients with HSV encephalitis.RESULTS: Sixty-six participants reported a total of 76 data sets for panel 1, and 71 reported 78 data sets for panel 2. The majority of the participants employed qualitative 'in-house' polymerase chain reaction (PCR) methods, either in a single, nested or semi-nested format. For panel 2, 9 laboratories reported use of 'real-time' PCR in contrast to 3 for panel 1. Three laboratories submitted quantitative results on both panels. Thirty percent of the data sets had correct results for the entire panel 1. In 6 data sets (8%) a total of 11 false positive results were reported. For panel 2, 28% of the data sets had correct result. Nineteen false positive results were reported in 14 data sets (18%), but most of the incorrect results reflected a lack of test sensitivity.CONCLUSIONS: The relatively high frequency of false positive results and the large number of false-negative results, albeit at low copy number, stress the need for improvement in the quality of HSV NAT and for external quality control programmes.

AB - BACKGROUND: There is an increasing awareness of the need for external quality control of diagnostic virology.OBJECTIVES: To assess the quality of nucleic acid amplification tests (NAT) of herpes simplex within Europe.STUDY DESIGN: Herpes simplex virus (HSV) proficiency panels were produced at the Swedish Institute for Infectious Disease Control on behalf of the European Union Concerted Action for Quality Control of Nucleic Acid Amplification in 1999 and 2000. Nine reference laboratories evaluated the production process. Each panel consisted of 12 coded samples with various concentrations of inactivated, freeze-dried HSV type 1 (HSV-1), and HSV type 2 (HSV-2), or negative controls. Positive samples included HSV-1 and HSV-2 in a range of concentrations (2 x 10(2) to 2 x 10(7) genome copies per ml) similar to those found in cerebrospinal fluids from patients with HSV encephalitis.RESULTS: Sixty-six participants reported a total of 76 data sets for panel 1, and 71 reported 78 data sets for panel 2. The majority of the participants employed qualitative 'in-house' polymerase chain reaction (PCR) methods, either in a single, nested or semi-nested format. For panel 2, 9 laboratories reported use of 'real-time' PCR in contrast to 3 for panel 1. Three laboratories submitted quantitative results on both panels. Thirty percent of the data sets had correct results for the entire panel 1. In 6 data sets (8%) a total of 11 false positive results were reported. For panel 2, 28% of the data sets had correct result. Nineteen false positive results were reported in 14 data sets (18%), but most of the incorrect results reflected a lack of test sensitivity.CONCLUSIONS: The relatively high frequency of false positive results and the large number of false-negative results, albeit at low copy number, stress the need for improvement in the quality of HSV NAT and for external quality control programmes.

KW - False Negative Reactions

KW - False Positive Reactions

KW - Herpes Simplex

KW - Humans

KW - International Cooperation

KW - Laboratories

KW - Polymerase Chain Reaction

KW - Quality Assurance, Health Care

KW - Quality Control

KW - RNA, Viral

KW - Reference Standards

KW - Reproducibility of Results

KW - Sensitivity and Specificity

KW - Simplexvirus

U2 - 10.1016/S1386-6532(03)00003-9

DO - 10.1016/S1386-6532(03)00003-9

M3 - Article

C2 - 12957188

SN - 1386-6532

VL - 28

SP - 175

EP - 785

JO - Journal of Clinical Virology

JF - Journal of Clinical Virology

IS - 2

ER -

An international external quality assessment of nucleic acid amplification of herpes simplex virus

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