A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage

T Engel; B J Slotboom; N van Maarseveen; A A van Zwet; M H Nabuurs-Franssen; F Hagen

doi:10.1016/j.jhin.2017.07.017

A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage

T Engel
, B J Slotboom
, N van Maarseveen
, A A van Zwet
, M H Nabuurs-Franssen
, F Hagen^*

^*Corresponding author for this work

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

Abstract

OBJECTIVE: A multiplex extended-spectrum beta-lactamase-producing Enterobacteriaceae (ESBL-E) quantitative polymerase chain reaction (qPCR), performed directly on rectal swabs, was compared with a culture-based protocol to study the discrepancies between the two methods, and identify existing challenges to apply this assay in routine clinical practice. The secondary objective was to assess the performance of the qPCR.

MATERIALS AND METHODS: In two Dutch teaching hospitals, 573 rectal swabs were collected prospectively. Culture with additional testing with the Check-MDR CT103XL (Check-Points) was compared with the Check-Direct ESBL Screen for BD MAX (Check-Points), which detects the presence of the ESBL gene families CTX-M1, CTX-M2, CTX-M9 and SHV2/5-ESBL. The culture-based protocol (with Brilliance agar) was considered as the gold standard to assess the performance of the qPCR.

RESULTS: Of the 573 rectal swabs, 74 (12.9%) were culture-positive. Eighty-four (14.7%) were qPCR-positive. There were eight culture-positive/qPCR-negative discrepancies and 18 culture-negative/qPCR-positive discrepancies. Sensitivity and specificity of qPCR vs culture were 87.7% [95% confidence interval (CI) 79.7-95.7] and 96.3% (95% CI 94.6-98.0), respectively.

CONCLUSION: The Check-Direct ESBL Screen for the BD MAX is an easy-to-perform, quick molecular diagnostic test with the potential to significantly speed up screening for rectal ESBL-E carriage. Discrepancies were observed between the culture-based protocol and the qPCR in 4.5% of tested samples. Existing challenges for implementing qPCR are its limited sensitivity, the need for thorough knowledge of the local ESBL-E genes, and interpretation of culture-negative but qPCR-positive samples. It is believed that the limited sensitivity of qPCR could be optimized by including blaTEM as a molecular target, and improving the limit of detection.

Original language	English
Pages (from-to)	247-253
Number of pages	7
Journal	The journal of Hospital Infection
Volume	97
Issue number	3
DOIs	https://doi.org/10.1016/j.jhin.2017.07.017
Publication status	Published - Nov 2017
Externally published	Yes

Keywords

Bacteriological Techniques/methods
Carrier State/diagnosis
Enterobacteriaceae Infections/diagnosis
Hospitals
Humans
Mass Screening/methods
Molecular Diagnostic Techniques/methods
Netherlands
Prospective Studies
Rectum/microbiology
Sensitivity and Specificity
Time Factors
beta-Lactamases/genetics

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10.1016/j.jhin.2017.07.017

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Engel, T., Slotboom, B. J., van Maarseveen, N., van Zwet, A. A., Nabuurs-Franssen, M. H., & Hagen, F. (2017). A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage. The journal of Hospital Infection, 97(3), 247-253. https://doi.org/10.1016/j.jhin.2017.07.017

@article{f7bf192b3fda4a6a9c85ef461e97f3ce,

title = "A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage",

abstract = "OBJECTIVE: A multiplex extended-spectrum beta-lactamase-producing Enterobacteriaceae (ESBL-E) quantitative polymerase chain reaction (qPCR), performed directly on rectal swabs, was compared with a culture-based protocol to study the discrepancies between the two methods, and identify existing challenges to apply this assay in routine clinical practice. The secondary objective was to assess the performance of the qPCR.MATERIALS AND METHODS: In two Dutch teaching hospitals, 573 rectal swabs were collected prospectively. Culture with additional testing with the Check-MDR CT103XL (Check-Points) was compared with the Check-Direct ESBL Screen for BD MAX (Check-Points), which detects the presence of the ESBL gene families CTX-M1, CTX-M2, CTX-M9 and SHV2/5-ESBL. The culture-based protocol (with Brilliance agar) was considered as the gold standard to assess the performance of the qPCR.RESULTS: Of the 573 rectal swabs, 74 (12.9\%) were culture-positive. Eighty-four (14.7\%) were qPCR-positive. There were eight culture-positive/qPCR-negative discrepancies and 18 culture-negative/qPCR-positive discrepancies. Sensitivity and specificity of qPCR vs culture were 87.7\% [95\% confidence interval (CI) 79.7-95.7] and 96.3\% (95\% CI 94.6-98.0), respectively.CONCLUSION: The Check-Direct ESBL Screen for the BD MAX is an easy-to-perform, quick molecular diagnostic test with the potential to significantly speed up screening for rectal ESBL-E carriage. Discrepancies were observed between the culture-based protocol and the qPCR in 4.5\% of tested samples. Existing challenges for implementing qPCR are its limited sensitivity, the need for thorough knowledge of the local ESBL-E genes, and interpretation of culture-negative but qPCR-positive samples. It is believed that the limited sensitivity of qPCR could be optimized by including blaTEM as a molecular target, and improving the limit of detection.",

keywords = "Bacteriological Techniques/methods, Carrier State/diagnosis, Enterobacteriaceae Infections/diagnosis, Hospitals, Humans, Mass Screening/methods, Molecular Diagnostic Techniques/methods, Netherlands, Prospective Studies, Rectum/microbiology, Sensitivity and Specificity, Time Factors, beta-Lactamases/genetics",

author = "T Engel and Slotboom, \{B J\} and \{van Maarseveen\}, N and \{van Zwet\}, \{A A\} and Nabuurs-Franssen, \{M H\} and F Hagen",

note = "Publisher Copyright: {\textcopyright} 2017 The Healthcare Infection Society",

year = "2017",

month = nov,

doi = "10.1016/j.jhin.2017.07.017",

language = "English",

volume = "97",

pages = "247--253",

journal = "The journal of Hospital Infection",

issn = "0195-6701",

publisher = "W.B. Saunders Ltd",

number = "3",

}

Engel, T, Slotboom, BJ, van Maarseveen, N, van Zwet, AA, Nabuurs-Franssen, MH & Hagen, F 2017, 'A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage', The journal of Hospital Infection, vol. 97, no. 3, pp. 247-253. https://doi.org/10.1016/j.jhin.2017.07.017

A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage. / Engel, T; Slotboom, B J; van Maarseveen, N et al.
In: The journal of Hospital Infection, Vol. 97, No. 3, 11.2017, p. 247-253.

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

TY - JOUR

T1 - A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage

AU - Engel, T

AU - Slotboom, B J

AU - van Maarseveen, N

AU - van Zwet, A A

AU - Nabuurs-Franssen, M H

AU - Hagen, F

PY - 2017/11

Y1 - 2017/11

N2 - OBJECTIVE: A multiplex extended-spectrum beta-lactamase-producing Enterobacteriaceae (ESBL-E) quantitative polymerase chain reaction (qPCR), performed directly on rectal swabs, was compared with a culture-based protocol to study the discrepancies between the two methods, and identify existing challenges to apply this assay in routine clinical practice. The secondary objective was to assess the performance of the qPCR.MATERIALS AND METHODS: In two Dutch teaching hospitals, 573 rectal swabs were collected prospectively. Culture with additional testing with the Check-MDR CT103XL (Check-Points) was compared with the Check-Direct ESBL Screen for BD MAX (Check-Points), which detects the presence of the ESBL gene families CTX-M1, CTX-M2, CTX-M9 and SHV2/5-ESBL. The culture-based protocol (with Brilliance agar) was considered as the gold standard to assess the performance of the qPCR.RESULTS: Of the 573 rectal swabs, 74 (12.9%) were culture-positive. Eighty-four (14.7%) were qPCR-positive. There were eight culture-positive/qPCR-negative discrepancies and 18 culture-negative/qPCR-positive discrepancies. Sensitivity and specificity of qPCR vs culture were 87.7% [95% confidence interval (CI) 79.7-95.7] and 96.3% (95% CI 94.6-98.0), respectively.CONCLUSION: The Check-Direct ESBL Screen for the BD MAX is an easy-to-perform, quick molecular diagnostic test with the potential to significantly speed up screening for rectal ESBL-E carriage. Discrepancies were observed between the culture-based protocol and the qPCR in 4.5% of tested samples. Existing challenges for implementing qPCR are its limited sensitivity, the need for thorough knowledge of the local ESBL-E genes, and interpretation of culture-negative but qPCR-positive samples. It is believed that the limited sensitivity of qPCR could be optimized by including blaTEM as a molecular target, and improving the limit of detection.

AB - OBJECTIVE: A multiplex extended-spectrum beta-lactamase-producing Enterobacteriaceae (ESBL-E) quantitative polymerase chain reaction (qPCR), performed directly on rectal swabs, was compared with a culture-based protocol to study the discrepancies between the two methods, and identify existing challenges to apply this assay in routine clinical practice. The secondary objective was to assess the performance of the qPCR.MATERIALS AND METHODS: In two Dutch teaching hospitals, 573 rectal swabs were collected prospectively. Culture with additional testing with the Check-MDR CT103XL (Check-Points) was compared with the Check-Direct ESBL Screen for BD MAX (Check-Points), which detects the presence of the ESBL gene families CTX-M1, CTX-M2, CTX-M9 and SHV2/5-ESBL. The culture-based protocol (with Brilliance agar) was considered as the gold standard to assess the performance of the qPCR.RESULTS: Of the 573 rectal swabs, 74 (12.9%) were culture-positive. Eighty-four (14.7%) were qPCR-positive. There were eight culture-positive/qPCR-negative discrepancies and 18 culture-negative/qPCR-positive discrepancies. Sensitivity and specificity of qPCR vs culture were 87.7% [95% confidence interval (CI) 79.7-95.7] and 96.3% (95% CI 94.6-98.0), respectively.CONCLUSION: The Check-Direct ESBL Screen for the BD MAX is an easy-to-perform, quick molecular diagnostic test with the potential to significantly speed up screening for rectal ESBL-E carriage. Discrepancies were observed between the culture-based protocol and the qPCR in 4.5% of tested samples. Existing challenges for implementing qPCR are its limited sensitivity, the need for thorough knowledge of the local ESBL-E genes, and interpretation of culture-negative but qPCR-positive samples. It is believed that the limited sensitivity of qPCR could be optimized by including blaTEM as a molecular target, and improving the limit of detection.

KW - Bacteriological Techniques/methods

KW - Carrier State/diagnosis

KW - Enterobacteriaceae Infections/diagnosis

KW - Hospitals

KW - Humans

KW - Mass Screening/methods

KW - Molecular Diagnostic Techniques/methods

KW - Netherlands

KW - Prospective Studies

KW - Rectum/microbiology

KW - Sensitivity and Specificity

KW - Time Factors

KW - beta-Lactamases/genetics

U2 - 10.1016/j.jhin.2017.07.017

DO - 10.1016/j.jhin.2017.07.017

M3 - Article

C2 - 28743503

SN - 0195-6701

VL - 97

SP - 247

EP - 253

JO - The journal of Hospital Infection

JF - The journal of Hospital Infection

IS - 3

ER -

Engel T, Slotboom BJ, van Maarseveen N, van Zwet AA, Nabuurs-Franssen MH, Hagen F. A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage. The journal of Hospital Infection. 2017 Nov;97(3):247-253. doi: 10.1016/j.jhin.2017.07.017

A multi-centre prospective evaluation of the Check-Direct ESBL Screen for BD MAX as a rapid molecular screening method for extended-spectrum beta-lactamase-producing Enterobacteriaceae rectal carriage

Abstract

Keywords

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