How to: diagnose infection caused by Clostridium difficile

Accepted Manuscript How to: Diagnose infection caused by Clostridium difficile Cécile Gateau, Jeanne Couturier, John Coia, Frédéric Barbut PII:

S1198-743X(17)30678-X

DOI:

10.1016/j.cmi.2017.12.005

Reference:

CMI 1147

To appear in:

Clinical Microbiology and Infection

Received Date: 1 October 2017 Revised Date:

30 November 2017

Accepted Date: 7 December 2017

Please cite this article as: Gateau C, Couturier J, Coia J, Barbut F, How to: Diagnose infection caused by Clostridium difficile, Clinical Microbiology and Infection (2018), doi: 10.1016/j.cmi.2017.12.005. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.

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How to: diagnose infection caused by Clostridium difficile

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Cécile Gateau1, Jeanne Couturier1,2, John Coia3,4, Frédéric Barbut1,2,4

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Author’s affiliation:

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Antoine, 34 rue Crozatier, 75012 Paris, France

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EA4065, Université Paris Descartes, Paris, France

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Scottish Microbiology Reference Laboratories, Glasgow, Scotland

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European study group on Clostridium difficile

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National Reference Laboratory for C. difficile, Assistance Publique-Hôpitaux de Paris, Hôpital Saint-

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Contact information / corresponding author:

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Pr Frédéric Barbut

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[email protected],

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National Reference Laboratory for C. difficile,

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Hôpital Saint-Antoine, AP-HP

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34 rue Crozatier,

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75012 Paris, France.

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Tel: 33 1 49 28 30 11

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Fax: 33 1 49 28 30 09

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Statement indicating:

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Length of the abstract: 250 words

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Length of the paper (excluding abstract and references): 3441 words

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ACCEPTED MANUSCRIPT Abstract

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Background: Clostridium difficile is recognized as the major agent responsible for nosocomial

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diarrhoea. In the context of recent increase in the incidence and severity of CDI, an accurate

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diagnosis is essential for optimal treatment and prevention, but continues to be challenging.

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Aims: The present article reviews each key step of CDI diagnosis including stool selection, methods

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and strategies used, and interpretation of the results.

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Sources: The most recent guidelines for CDI diagnosis published by scientific societies were

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reviewed.

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Content: CDI diagnosis is based on clinical presentation and laboratory tests confirming the

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presence of toxigenic strain or toxins in stools. Stool selection is crucial and can be improved by

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implementing rejection criteria and strict policy for appropriate testing. Multiple laboratory tests

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detecting different targets (free toxin or presence of a potentially toxigenic strain) are commercially

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available. However, none of these tests combine high sensitivity and specificity to diagnose CDI, low

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hands-on time and low cost. An optimized diagnosis can be achieved by implementing a 2- or 3-step

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algorithm. Algorithms currently recommended by the ESCMID consist in a screening test with high

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sensitivity followed with a more specific test to detect free toxins. Presence of free toxins in stools

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has been shown to better correlate with severe outcome whereas nucleic acid amplification tests

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(NAAT) may lead to an over-diagnosis by detecting asymptomatic carriers of a toxigenic strain.

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Implication: To date, no single test can accurately diagnose CDI. Guidelines from the ESCMID

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recommend a 2 or 3-step algorithm for an optimal CDI detection.

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Keywords: Clostridium difficile, diagnostic methods, nucleic acid amplification test, glutamate

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dehydrogenase, toxins, diarrhoea, colitis

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Clostridium difficile is an anaerobic Gram-positive spore-forming bacillus responsible for a

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wide spectrum of clinical symptoms ranging from a mild self-limited diarrhea to pseudomembranous

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colitis (PMC), toxic megacolon, septic shock and possible death [1–5]. Risk factors for C. difficile

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infections (CDI) include age above 65 years, previous hospitalization, recent antibiotic therapy (in

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particular

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fluoroquinolones), immunosuppression and proton pump inhibitors [3,6]. Asymptomatic carriage is

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observed in 3% of patients on admission to hospital [7]. This frequency is higher among healthy

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neonates (30%-50%) and hospitalized patients (20 to 30%) [8]. Treatment and isolation of

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asymptomatic carriers are currently not recommended despite some evidence that they could play a

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role in C. difficile transmission [7,9]. In the U.S.A, C. difficile is the leading cause of healthcare-

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associated infections with more than 453 000 CDI per year, leading to 29 600 deaths [10]. In Europe,

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the estimated number of healthcare-associated CDI is 126 000 per year with a 3% attributable

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mortality [11]. C. difficile is also recognized as a major pathogen in the community despite substantial

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underdiagnosis [12]. The incidence of CDI has been increasing worldwide partly due to the

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emergence of an epidemic strain (NAP1/027/BI) responsible for large outbreaks of severe CDI in the

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last few years [13,14]. This hypervirulent clone is now endemic in Europe and the United States,

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despite large variations across countries or states [10,15]. A rapid and accurate diagnosis is essential

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to guide the treatment and to prevent transmission. It has been shown that rapid diagnosis impacts

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positively on the patient’s care by reducing delays in initiation of isolation and treatment for

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confirmed CDI cases. A negative test will also result in rapid discontinuation of empirical therapy and

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isolation [16,17]. Reliable data are also crucial for monitoring CDI incidence over time and

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comparison between different healthcare facilities. The purpose of this article is to review the

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methods and strategies currently available for CDI diagnosis and to highlight essential factors of CDI

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testing optimization.

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cephalosporins,

amoxicillin-clavulanate,

clindamycin,

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How to define a case of C. difficile infection? Only toxigenic strains, producing toxin A and/or B, are pathogenic [18]. According to the

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European Society of Clinical Microbiology and Infectious Diseases (ESCMID) guidelines, a CDI is

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defined as “(i) a clinical picture compatible with CDI and microbiological evidence of toxin A and/or

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toxin B producing C. difficile in stool without evidence of another cause of diarrhea or (ii) patient with

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PMC” [5]. A similar definition is given by the Society for Healthcare Epidemiology of America (SHEA)

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and the Infectious Diseases Society of America (IDSA): “A case of CDI is defined by the presence of

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symptoms (usually diarrhea) and either a stool test positive for C. difficile toxins or toxigenic C.

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difficile, or colonoscopic or histopathologic findings revealing PMC ”[19].

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How to select stool samples?

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Stool selection is essential since currently available tests do not accurately distinguish CDI

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from asymptomatic carriage of toxigenic C. difficile. This selection can be improved by implementing

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rejection criteria and a strict policy for appropriate testing. Continuous education of physicians and

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nurses along with monitoring and feedback are also necessary to reduce inappropriate testing [20].

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Only liquid or unformed stools, i.e. specimens taking the shape of the container, should be

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processed to avoid the identification of asymptomatic carriers. Because of insufficient volume, stool

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swabs cannot be used for toxin tests. However, swabs can be analyzed by culture or nucleic acid

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amplification tests (NAAT) for epidemiological studies or in case of a patient presenting with an ileus.

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For optimal recovery, stool specimens should be cultured within two hours after collection and must

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be preserved in a leak-proof container. Beyond this time, even if some spores can survive at 4°C, the

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number of viable C. difficile vegetative cells will significantly decrease. For toxin assay, stools can be

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stored at 4°C for a maximum of 3 days. If testing is delayed, specimens have to be frozen at -80°C

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[21,22]. Stool samples from children less than 3 years old should only be tested in specific cases (e.g

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neonates with Hirschprung disease or suspicion of an outbreak) because asymptomatic carriage is

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common in this population [23].

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Repeated testing should be discouraged [24] because of a low diagnostic gain (defined as the

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rate of negative samples that convert to positive) [25,26]. In addition, this practice increases the

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likelihood of false positive results due to lack of specificity of the methods [27]. This practice was

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frequent when EIA (Enzyme Immunoassay) for toxins was used as a stand-alone test to overcome the

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lack of sensitivity of these tests. If the new proposed algorithms are used (see section “which

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algorithm to use”), then a negative result with a screening test can reliably rule out the diagnosis of

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CDI due to the high negative predictive value (NPV) at low disease prevalence. However, in cases of

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outbreak situations where CDI prevalence is higher, the NPV of the algorithm will decrease, and a

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repeat sample in cases of ongoing clinical suspicion may be justified.

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Clinical cure is defined by the resolution of the symptoms. A “test-of-cure” is not

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recommended [28], since toxins and/or spores can persist in stools up to 6 weeks, despite symptom

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resolution [29].

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Stool samples should be taken prior to initiation of treatment to avoid false negative results.

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Indeed, in a prospective study including 51 patients with CDI, Sunkesula et al. [30] determined the

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conversion time of positive to negative test results after initiation of treatment. They showed that

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14%, 35%, and 45% of PCR positive tests are converted to negative after 1, 2, and 3 days of

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treatment, respectively. Physicians should be aware that any empirical therapy for suspected CDI

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started before stool collection can lead to a false-negative test result.

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What are the different diagnostic methods?

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Several laboratory tests, detecting different targets, are currently available to diagnose CDI

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(Fig 1). These tests detect either free toxins in stools (enzyme immunoassay [EIA], stool cytotoxicity

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assay [CTA]), the presence of C. difficile (EIA for glutamate dehydrogenase, [GDH]), or the presence of

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a toxigenic C. difficile strain (toxigenic culture [TC], nucleic acid amplification tests [NAAT]). Stool CTA

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and TC are considered as the gold-standard methods for detecting toxins or a toxigenic strain,

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respectively. Paradoxically, neither are routinely used because of technical issues and long

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turnaround time.

TC is a two-step method where C. difficile strains are first isolated on a selective medium [31–

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33] and then tested for their ability to produce toxins in vitro. Different selective media are available

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and they usually derive from the cycloserine cefoxitin fructose agar (CCFA) medium initially described

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by George et al. [31]. Subsequently, additive such as sodium taurocholate or lysozyme were added

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to stimulate germination and to enhance recovery. Chromogenic media have also been developed:

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they were shown to be as sensitive as other selective media, yielding identification within 24 h of

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incubation [32]. Plates are incubated in an anaerobic atmosphere for 48h at 36°C + 1°C. Strain

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identification can be performed using gallery strips, gas liquid chromatography, latex agglutination

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for GDH or matrix assisted laser desorption ionization-time-of-flight [MALDI-TOF] mass spectrometry.

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After isolation of a strain, its pathogenic potential is ascertained by testing for its in vitro toxin

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production directly from a suspension of colonies or from the broth supernatant of bacterial growth.

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TC is considered as the reference method to detect toxigenic C. difficile and remains a gold standard

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for evaluating new molecular methods. Although the turnaround time of this method is too long for

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routine diagnosis (2 to 5 days), culture is essential for subsequent typing, molecular analysis and

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determination of antimicrobial susceptibility.

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GDH is a metabolic enzyme expressed by all C. difficile strains. It can be detected by immuno-

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enzymatic (ELISA) or immuno-chromatographic assays. A positive result only indicates the presence

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of C. difficile, without predicting the ability of the strain to produce toxins. Different guidelines now

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proposed GDH EIA tests as a screening method for CDI diagnosis. Because of its high NPV (80.0%-

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100% [reviewed in [28] and [34]]), a negative test for GDH will generally rule out the infection.

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However, a NPV should be interpreted with caution and strongly depends on the prevalence of the

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disease: with a NPV of 99% and a CDI prevalence of 10%, one positive stool out of ten will be

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discarded if GDH is used as a screening test. A positive GDH result has to be confirmed by a second

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more specific test detecting toxins. CTA is considered as the reference method for detecting free toxins (mainly toxin B) in stools.

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This method consists in inoculating a stool filtrate on a cell culture and observing a specific cytopathic

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effect (CPE) (cell rounding) after 1 or 2 days of incubation at 36 + 1°C. Specificity of the CPE is

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assessed by neutralization with antisera directed against C. difficile toxin B or against C. sordellii

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toxins, which share the same antigens. In a large prospective study in the United Kingdom, positivity

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of stool CTA was shown to better correlate with clinical outcome than presence of toxigenic C.

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difficile [14]. Despite good sensitivity and specificity [35] and low cost of CTA, this method is currently

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used by a very limited number of laboratories because of lack of standardization (type of cells used,

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dilution of stool samples, incubation period) and long turn-around time.

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EIA mainly detect both toxins A and B (with or without differentiation) using monoclonal or polyclonal

antibodies

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micro-well immuno-enzymatic

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immuno-

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chromatographic/lateral flow membrane devices. Many commercial EIAs are available. They provide

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rapid results and are easy to use. Nevertheless, many studies highlighted their lack of sensitivity

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(ranging from 29% to 86% reviewed in [28]) compared to CTA, precluding their use as stand-alone

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tests for CDI diagnosis.

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NAATs are based on real-time PCR, loop isothermal amplification or microarray technologies.

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Since the first FDA-approved test in 2009, new tests are regularly marketed (Table I). Some platforms

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are designed for low volume laboratories or point-of-care, whereas others are more suitable for high

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throughput testing. NAATs detect a large variety of targets including tcdB, tcdA, ∆117 deletion in tcdC

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(as a surrogate marker of the 027 epidemic strain) or binary toxin (cdt) genes. Some test systems

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combine detection of toxigenic strains of C. difficile with tests for other gastrointestinal pathogens in

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a syndromic approach [36]. Other characteristics like DNA extraction method, use of internal

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controls, manual assays or fully automated systems, must be considered when choosing a molecular

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method. NAATs are very sensitive (average sensitivity of 96% (95% CI = 0.93-0.98) compared to TC

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[37]) and have a high NPV. Like TC, the use of NAAT can lead to overdiagnosis of CDI due to

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asymptomatic carriage of toxigenic strain or inappropriate test ordering (e.g. patient without

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diarrhea). Indeed, these methods do not detect free toxins in the stool but only the genes encoding

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the toxins. In addition, one potential concern is genetic variation in tcdB or tcdA genes [38–40] that

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could lead to false negative results. As a result, the European Society of Clinical Microbiology and

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Infectious Diseases (ESCMID) guidelines do not recommend using NAAT as a stand-alone test for C.

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difficile diagnosis but rather to use NAAT as a screening test given its high negative predictive value

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for CDI. Then, a more specific toxin test will be used to identify patients most likely to have CDI.

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Results of NAATs can be achieved in one hour but they remain more expensive than TC or antigen-

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based assays. This is often a major obstacle to implement this technique as a screening method in a

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laboratory.

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Which strategy to implement?

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The optimal approach for detection of CDI is still matter of debates [41]. According the

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ESCMID, no single test can be recommended as a stand-alone test for diagnosing CDI, given their low

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positive predictive value (PPV) at a low CDI prevalence. Therefore, to optimize CDI diagnosis, two-

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step algorithms are currently recommended [28](fig.2). The first test should have a high NPV (i.e. a

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highly sensitive test) that reliably classifies patients as non-CDI; it can either be a GDH EIA or NAAT.

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The choice between both assays depends on the local organization, financial constraints and stool

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numbers tested per day. In case of a positive result, a second test with a high positive predictive

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value (PPV) (i.e. a highly specific test such as toxin A/B EIA) should be used. Patients with a positive

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second test can be reliably classified as CDI. Patients with a negative second test for toxins should be

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clinically evaluated: they can be either truly infected (with toxin level below the threshold detection

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of the toxin EIA assay) or carriers of a toxigenic strain (Fig. 2) [28]. If GDH was the initial test, then an

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optional third step can be performed by TC or NAAT to discern toxigenic from non-toxigenic strains.

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An alternative algorithm is to simultaneously detect GDH and toxins A and B by EIA. Different

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tests are now commercially available (C. diff Quik Chek Complete, TechLab, Alere; CERTEST

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Clostridium difficile GDH+toxin A+B, Theradiag; C. difficile GDH-toxins A-B, MonlabTest, Orgentec).

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The diagnosis of CDI can be reliably excluded in case of negative results for both GDH and toxins, and

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conversely patients with both positive GDH and toxin results can be classified as CDI. Samples with

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GDH-negative and toxin-positive results are rarely observed and need to be retested. In case of GDH-

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positive samples that are negative for both toxins, NAATs are optionally recommended by the

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ESCMID in order to determine whether a toxigenic C. difficile strain is present.

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How to interpret the results?

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The diagnosis of CDI relies on clinical evidence in association with laboratory tests. There is

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general agreement across international guidelines that EIA for toxins should not be used as a stand-

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alone test, while the debate regarding the clinical interpretation of the presence of a toxigenic strain

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without detectable toxins in stools is ongoing. A large observational study of more than 12 000

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patients with diarrhea was conducted in the UK [14]. Patients with a positive CTA assay had

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increased mortality and higher blood leukocyte counts compared to patients with diarrhea but

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negative for C. difficile, whereas those with detection of toxigenic C. difficile without free toxin (TC

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positive, CTA negative) did not. The authors concluded that detection of free toxin best correlated

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with poor clinical outcome and best defined CDI. These results were confirmed in a prospective

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observational cohort study at a single center in US, showing that patients positive for NAAT and toxin

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had more complications, a higher fecal lactoferrin level and a higher blood leukocyte count than

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patients positive for NAAT but negative for toxins [42]. Patients with positive TC but negative CTA are

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usually classified as potential C. difficile excretors (i.e., asymptomatic carriers with diarrhea not due

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to CDI) [14,42]; the isolation of these patients is recommended by some to prevent cross-

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transmission but this should be assessed case by case. In fact, a negative test for toxin in stool

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sample does not completely rule out the diagnosis of CDI. It has been shown that 11% of diarrheic

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patients harboring toxigenic strains of C. difficile but without detectable toxin in stools have

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pseudomembranes during endoscopic examination, suggesting that some CDI cases may be missed

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by reliance on toxin tests only [43].

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How do European countries perform?

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Underdiagnosis of CDI is a major issue in Europe. In a Spanish point-prevalence study, 66% of

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patients with CDI were undiagnosed or misdiagnosed because of lack of clinical suspicion (47.6%) or a

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lack of sensitivity of the diagnostic methods (19%) [44]. The European multicenter point prevalence

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study (EUCLID) conducted in 482 healthcare facilities from 20 countries indicated that 23% of

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samples positive for C. difficile were not diagnosed by participating laboratories due to a lack of

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clinical suspicion and that 1.5% were misdiagnosed due to false negative results. These results

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highlight the substantial burden of undetected CDI cases in Europe, which is likely to hamper control

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measures [15].

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A survey of diagnostic capacity was performed in Europe in 2011 and 2014 under the

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auspices of the European Clostridium difficile Infection Surveillance Network [45]. In 2011, 126

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laboratories from 31 countries completed a survey on local diagnostics. In 2014, a follow-up study

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was carried out by 84 of these 126 laboratories (67%) from 26 countries. The use of an optimal

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strategy (namely a 2-step algorithm as defined by the ESCMID guidelines) increased from 19% to

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46% [45]. The indications for CDI diagnostics reported in 2011 were on all stool samples in 2%, on all

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diarrheal stool specimens in 28%, in case of antibiotic-associated diarrhea in 50%, in cases of

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healthcare-associated diarrhea in 32%, and only upon physician’s request in 33%. In 2014, an

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improvement has been observed in indications for sending samples including an increased use of the

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Bristol stool scale to assess stool consistency for sample selection, an increased awareness from

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physicians for testing patients previously not monitored for CDI (e.g. outpatients, high-risk

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populations) and a better implementation of guidelines for sample selection (e.g. the three-day rule).

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In conclusion, the detection of C. difficile and its toxins should be carried out systematically in

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cases of healthcare-associated diarrhea or in case of any unexplained diarrhea. The implementation

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of an optimal diagnostic strategy based on a two-step algorithm provides a good trade-off between

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sensitivity and specificity for the CDI diagnostic and will allow a better management of the patients.

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ACCEPTED MANUSCRIPT Transparency declaration

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Gateau C. has nothing to disclose.

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Dr. Couturier reports non-financial support from Astellas, outside the submitted work.

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Dr. Coia has nothing to disclose.

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Dr. BARBUT reports grants, personal fees and non-financial support from Astellas, personal fees from

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Pfizer, grants and personal fees from Sanofi Pasteur, grants and non-financial support from Anios,

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grants, personal fees and non-financial support from MSD, grants from Biomérieux, grants from

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Quidel Buhlman, grants from Diasorin, grants from Cubist, grants from Biosynex, grants from

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GenePoc, outside the submitted work.

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Funding

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This study did not receive any external funding

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Acknowledgments

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The authors are grateful to the European Study Group on Clostridium difficile (ESGCD).

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ACCEPTED MANUSCRIPT Table 1: Classification of commercially available NAAT for C. difficile (not exhaustive).

Detection of a single target Method

Target

®

Illumigene C.difficile (Meridian Bioscience)

tcdA

®

AmpliVue (QUIDELMolecular)

RI PT

tcdA

Simplexa™ C.difficile Universal Direct (FOCUS Diagnostics)

tcdB

Portrait Toxigenic C.difficile Assay (Portrait, Great Basin)

COBAS™ Cdiff (Roche) Prodesse ProGastro Cd assay (Gen Probe) ®

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ICEPlex C.difficile Kit (PrimeraDax)

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BD MAX™ Cdiff (BD Diagnostics)

tcdB

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BD GeneOhm™ Cdiff Assay (BD Diagnostics)

tcdB

tcdB

tcdB

tcdB

tcdB

Detection of several targets

Method ®

EP

GenoType Cdiff (Hain Lifescience)

Target tcdA, tcdB, several deletions in tcdC (including ∆117) cdtA, cdtB, gyrA, tpi

®

AC C

IMDx C.difficile (IntelligentMDx)

tcdA, tcdB

®

Xpert C.difficile (Cepheid) ®

tcdB, cdt, deletion in position 117 in tcdC

Verigene C.difficile Test (Nanosphere)

tcdA, tcdB, binary toxin, deletion in position 117 in tcdC

RIDA GENE Clostridium difficile & Toxin A/B (R-biopharm)

tcdA, tcdB

®

®

Genspeed C.Diff Onestep (Genspeed Biotech)

gdh, tcdA, tcdB, binary toxin

®

Quidel Molecular Direct C.difficile Assay (Quidel Corporation)

tcdA, tdcB

ACCEPTED MANUSCRIPT Detection of several pathogens Method

Target

®

Seeplex Diarrhea ACE Detection (Seegene) ®

FilmArray Gastrointestinal Panel (Biomerieux)

®

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RIDA GENE Gastro Panel (R-biopharm)

9 bacteria (including C. difficile tcdA tcdB genes) 3 viruses 3 parasites 22 bacteria (including C. difficile tcdB gene) 4 viruses 20 bacteria (including C. difficile tcdA tcdB genes) 5 viruses 4 parasites 10 bacteria (including C. difficile tcdA tcdB genes) 5 viruses 4 parasites

RI PT

®

xTAG Gastrointestinal Pathogen Panel (Theradiag)

ACCEPTED MANUSCRIPT

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Fig.1: Advantages, disadvantages and targets of the different methods used for the diagnosis of CDI

TE D

CTA: Cytotoxicity assay; EIA: Enzyme immunoassay; GDH: Glutamate dehydrogenase; NAAT: Nucleic acid

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amplification test; NPV: Negative predictive value; TAT: Turnaround time; CDI: Clostridium difficile infection.

ACCEPTED MANUSCRIPT

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Fig. 2: Algorithms for the diagnosis of CDI (adapted from the ESCMID guidelines [28])

EIA: Enzyme immunoassay; GDH: Glutamate dehydrogenase; NAAT: Nucleic acid amplification test; CDI:

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Clostridium difficile infection ; TC: Toxigenic culture.