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Latent class analysis of diagnostic tests for adenovirus, Bordetella pertussis and influenza virus infections in German adults with longer lasting coughs

Published online by Cambridge University Press:  18 September 2015

C. SOBOTZKI ,
M. RIFFELMANN ,
N. KENNERKNECHT ,
C. HÜLSSE ,
M. LITTMANN ,
A. WHITE ,
R. VON KRIES  and
C. H. WIRSING VON KÖNIG
C. SOBOTZKI
Affiliation:
Institut für Soziale Pädiatrie und Jugendmedizin, Ludwig-Maximilians-Universität, München, Germany
M. RIFFELMANN
Affiliation:
Labor: Medizin Krefeld MVZ GmbH, Krefeld, Germany Institut für Hygiene und Labormedizin, HELIOS Klinikum Krefeld, Germany
N. KENNERKNECHT
Affiliation:
Institut für Hygiene und Labormedizin, HELIOS Klinikum Krefeld, Germany
C. HÜLSSE
Affiliation:
Landesamt für Gesundheit und Soziales des Landes Mecklenburg Vorpommern, Rostock, Germany
M. LITTMANN
Affiliation:
Landesamt für Gesundheit und Soziales des Landes Mecklenburg Vorpommern, Rostock, Germany
A. WHITE
Affiliation:
Trinity College Dublin, School of Computer Science and Statistics, Dublin, Ireland
R. VON KRIES
Affiliation:
Institut für Soziale Pädiatrie und Jugendmedizin, Ludwig-Maximilians-Universität, München, Germany
C. H. WIRSING VON KÖNIG*
Affiliation:
Labor: Medizin Krefeld MVZ GmbH, Krefeld, Germany
*
*Author for correspondence: Dr C. H. Wirsing von Koenig, Labor: Medizin Krefeld MVZ GmbH, Krefeld, Germany. (Email: carlheinz.wirsingvonkoenig@helios-kliniken.de)
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Summary

Laboratory tests in adult outpatients with longer lasting coughs to identify a potential causal pathogen are rarely performed, and there is no gold standard for these diagnostic tests. While the diagnostic validity of serological tests for pertussis is well established their potential contribution for diagnosing adenovirus and influenza virus A and B infections is unclear. A sentinel study into the population-based incidence of longer lasting coughs in adults was done in Rostock (former East Germany) and Krefeld (former West Germany). A total of 971 outpatients who consulted general practitioners or internists were included. Inclusion criteria were coughing for ⩾1 week and no chronic respiratory diseases. We evaluated the performance of polymerase chain reaction (PCR) as well as IgG and IgA serology, applying a latent class model for diagnosing infections with adenovirus, B. pertussis, and influenza virus A and B. The adult outpatients first sought medical attention when they had been coughing for a median of 3 weeks. In this situation, direct detection of infectious agents by PCR had a low sensitivity. Modelling showed that additional serological tests equally improved sensitivity and specificity for diagnosis for adenovirus, B. pertussis and influenza virus A and B infections. The combination of serology and PCR may improve the overall performance of diagnostic tests for B. pertussis and also for adenovirus, and influenza virus A and B infections.

Keywords

Adenovirusadultscoughinfluenza viruslatent class analysispertussis
Type
Original Papers
Information
Epidemiology & Infection , Volume 144 , Issue 4 , March 2016 , pp. 840 - 846
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Copyright
Copyright © Cambridge University Press 2015 

INTRODUCTION

With the advent of molecular methods in diagnostic virology, real-time polymerase chain reaction (PCR) is regarded as the method of choice for diagnosing viral respiratory diseases such as influenza A and B and adenovirus infections [Reference Qu1]. In adult outpatients, however, symptoms may persist for a lengthy period before medical attention is sought, and consequently, even if attempted, the sensitivity of direct detection of viruses may be not sufficiently high. For infections with Bordetella pertussis in adults, various studies have demonstrated that the sensitivity of Bordetella PCR was well below 10% and thus, serology has been the mainstay for diagnosing these infections [Reference von Konig2]. As no accepted ‘gold standard’ exists for these infections, latent class analysis (LCA) has been successfully applied to estimate the sensitivities and specificities of PCR and serology for pertussis diagnosis [Reference Baughman3]. LCA is a well-documented and statistically valid tool in absence of a gold standard [Reference Baughman3, Reference Rutjes4]. Moreover, the characteristics of this method have been extensively studied in comparison with estimates where a gold standard was available [Reference Rutjes4].

We used a sentinel study into longer lasting cough in adults with almost 1000 patients in two German cities to study the application of the latent class model for the diagnosis of pertussis and to extend it to the diagnosis of adenovirus as well as influenza virus A and B infections in order to evaluate the relative role of viral serology in this outpatient population.

PATIENTS AND METHODS

Patients were recruited from general practitioners (GPs) and internists, who were active in general internal medicine (Allgemeinärztlich tätige Internisten) (summarized as GPs) in Krefeld (former West Germany) and Rostock (former East Germany). Between 2001 and 2004 a total of 971 patients were included in the study. The study had 21 sentinels in Rostock and 14 in Krefeld. The 21 sentinels in Rostock treated 34·2% of all patients in Rostock and the 14 sentinels in Krefeld treated 19·2% of patients there. This study was approved by the ethical committees of the medical boards in Krefeld (Ärztekammer Nordrhein) and Rostock (Ärztekammer Mecklenburg-Vorpommern).

Inclusion criteria. Adult patients with a cough of ⩾7 days' duration were eligible for inclusion. Patients treated for chronic respiratory diseases such as chronic obstructive pulmonary disease, and patients participating in other studies were excluded. Clinical data about symptomatology, other diseases, contacts, professional background, duration of coughing and days off work were collected by two questionnaires. The first questionnaire asked about the duration of coughing before the first visit, for various other symptoms, for a history of similar episodes and for a contact anamnesis.

A total of 971 patients were included (455 from Rostock, 516 from Krefeld). Sixty-seven per cent were female (n = 650) and 33% were male (n = 221). The female:male ratio in Rostock was 71:29, and in Krefeld 65:35 (P > 0·2). The age distribution of all patients is given in Figure 1.

Fig. 1. Age distribution of study patients.

A total of 934 patients reported the duration of coughing symptoms before the first visit. For estimation of the mean time of symptoms before seeking medical attention we assumed that a total of 80 patients (8·5%) reporting symptoms for >3 months (12 weeks) would suffer from chronic coughing, and these were excluded from estimating the mean time before the first visit. Another 14 patients (1·5%) reported symptoms for <7 days (inclusion criterion) and these were also excluded from analysis.

Diagnostic procedures. A nasopharyngeal swab, pharyngeal washing and a peripheral blood sample was taken from all patients at presentation at the sentinels. Nasopharyngeal swabs were immersed in modified Amies medium with charcoal. Pharyngeal washings were sampled into a sterile tube. All samples were transported at ambient temperature to the central laboratory (Krefeld).

Laboratory tests. Nasopharyngeal swabs were tested for Bordetella DNA by real-time PCR targeting IS481 (B. pertussis), and IS1001 (B. parapertussis) [Reference Riffelmann5]. Pharyngeal washings were tested for adenovirus DNA, and influenza viruses A and B RNA by an in-house real-time PCR. For adenovirus PCR, a 131 nt fragment from the hexon gene of human adenovirus type 2, belonging to adenovirus species C, was amplified using TaqMan primers and probes and the amplification was performed on a 7500 RT–PCR system (ABI Biosystems, USA) [Reference Heim6]. For influenza A virus a 101 nt fragment from the M gene was amplified. The reverse primer was degenerated and a specific primer for the haemagglutinin variant H1sw was added. The probe was tagged with an amplifier molecule (ZNA; zipped nucleic acid). For influenza B virus a 89 nt fragment from the M gene was amplified. Amplification was done either on a 7500 RT–PCR or StepOne system (ABI Biosystems) [Reference Schulze7].

Serum samples were tested for IgG and IgA antibodies to adenovirus, for IgG and IgA antibodies to influenza virus A and B with a nucleoprotein as the respective antigen by micro-well ELISAs (all Virion Serion GmbH, Würzburg, Germany). IgG and IgA antibodies to pertussis toxin (PT) were measured by an in-house ELISA [Reference Wirsing von Konig8].

Interpretation of serology results. The commercial ELISAs measured antibodies quantitatively in arbitrary unit (AU/ml). The sensitivity of the commercial test systems was set to detect no antibodies to influenza virus A and B in healthy blood donors, irrespective of their immunization status to influenza virus. For antibodies to adenovirus, 95% of obviously healthy blood donors had no antibodies detected. Thus, we defined all detectable antibody levels as possibly indicative of a recent contact. For IgG anti-PT we followed the recommendations of the European reference laboratories [Reference Guiso9] and ⩾100 IU/ml was regarded as indicative of recent contact. For IgA anti-PT ⩾12 IU/ml was regarded as indicative of recent contact.

Statistical evaluation

We used LCA to assess diagnostic test accuracy [Reference Goodman10]. LCA hypothesizes the existence of one or more unobserved categorical variables to explain the relationships between a set of observed categorical variables. We treat the latent variable which corresponds to multiple positive diagnoses as the unobserved true disease status of the patients [Reference Rindskopf and Rindskopf11]. In the medical diagnosis context, the observed variables are, e.g. test results, usually dichotomized into a binary classification (positive and negative).

In the LCA model a posterior probability of the infections of interest is estimated with a frequentist expectation-maximization (EM) algorithm proposed by Qu et al. [Reference Qu, Tan and Kutner12]. For each possible test combination a response pattern depicting the posterior probability of being infected was calculated. If the posterior probability was >0·50, subjects were classified as infected [Reference Baughman3]. We repeated each LCA several times with different starting values for the EM algorithm in order to identify a stable pattern as proposed by Beath [Reference Beath13]. Sensitivity and specificity of the individual tests were estimated from the LCA. The sensitivity is the probability of the respective test to identify the subject correctly as infected under the condition that the subject is infected. Specificity on the other hand is the probability of correctly identifying a subject as not infected. Since the true infection status is unknown the latent class method constructs a hypothetical standard, and assesses the individual test's performance with respect to this hypothetical standard [Reference Beath13]. The 95% confidence limits were calculated using bootstrap methods [Reference Efron14].

As a sensitivity analysis we applied Bayesian LCA with non-informative priors via EM algorithms and Gibbs sampler [Reference White and Murphy15], a Markov chain Monte Carlo (MCMC) method. For the Gibbs sampler a sufficient burn-in was chosen and thinning was used to reduce autocorrelation between the observed output terms [16, Reference Plummer17]. An overview of the applied methods is described in Gentle et al. [Reference Gentle, Härdle and Mori18].

All analyses were performed with statistical software R 3.1.2 [19] and the add-on packages randomLCA [Reference Beath20] and BayesLCA [Reference White and Murphy15].

RESULTS

From the 934 patients, who reported the duration of coughing symptoms, we assumed that 80 had chronic cough (duration >12 weeks), and 14 reported coughing for <1 week. The remaining 840 patients reported coughing for a mean of 25·8 ± 17·6 days (3·7 weeks) and for a median of 21 days [95% confidence interval (CI) 7–63 days] before first seeking medical attention. No statistically significant difference was observed in the duration of symptoms between Krefeld and Rostock (P > 0·1).

Of the 971 study subjects, 948 patients had three tests for pertussis and 949 had three tests for adenovirus and influenza A and B, respectively.

Pertussis

A positive test result for pertussis was observed in 39 subjects (4·1%) by PT IgG, in 64 subjects (6·8%) by PT IgA and in 11 subjects (1·2%) by B. pertussis PCR (Table 1). Based on the LCA model a total of 23 subjects were classified as infected (Supplementary Table S1). According to this model, 22 (18 + 4) out of 23 (96%) could be detected with the test combination of PT IgG and PT IgA. Based on the LCA model the sensitivity for PT IgG was estimated as 1·00 (95% CI 0·99–1·00) followed by PT IgA 0·81 (95% CI 0·00–1·00) and B. pertussis PCR 0·19 (95% CI 0·04–0·53) (Table 2). The specificity was high in all tests. The data presented in Table 2 are based on the frequentist EM algorithm. A Bayesian EM algorithm and the Gibbs sampler yielded identical classification of pertussis infection (data not shown).

Table 1. Overall test results for polymerase chain reaction (PCR) and serology

PT IgG, IgG antibodies to pertussis toxin (PT); PT IgA, IgA antibodies to PT; Bp PCR, PCR for detecting Bordetella DNA; Adeno IgG, IgG antibodies to adenovirus; Adeno IgA, IgA antibodies to adenovirus; Adeno PCR, PCR for detecting adenovirus DNA; InfA IgG, IgG antibodies to influenza virus A; InfA IgA, IgA antibodies to influenza virus A; InfA PCR, PCR for detecting influenza virus A RNA; InfB IgG, IgG antibodies to influenza virus B; InfB IgA, IgA antibodies to influenza virus B; InfB PCR, PCR for detecting influenza virus B RNA.

Table 2. Estimated sensitivity and specificity of indicators of pertussis, adenovirus and influenza according to latent class analysis

Values in parentheses are 95% confidence intervals.

For abbreviations see Table 1.

Adenovirus

A positive test result for adenovirus was observed in 123 subjects (13·0%) by adenovirus IgG, in 176 subjects (18·5%) by adenovirus IgA and in 23 subjects (2·4%) by adenovirus PCR (Table 1). Based on the LCA model a total of 176 subjects were classified as infected (Supplementary Table S2). According to this model, all infected subjects could be detected by adenovirus IgA. The highest sensitivity was estimated as 1·00 (95% CI 0·99–1·00) for adenovirus IgA, 0·81 (95% CI 0·00–1·00) for adenovirus IgG and 0·19 (95% CI 0·04–0·53) for adenovirus PCR (Table 2). The specificity was high in all tests. The Bayesian EM algorithm and the Gibbs sampler yielded identical classification of adenovirus infection as the frequentist EM algorithm (data not shown).

Influenza A

A positive test result for influenza A was observed in 47 subjects (5·0%) by influenza A IgG, in 132 subjects (13·9%) by influenza A IgA and in 11 subjects (1·2%) by influenza A PCR (Table 1). Based on the LCA model a total of 47 subjects were classified as infected, all detected by influenza A IgG (Supplementary Table S3). Low sensitivity was estimated with 0·21 (95% CI 0·00–0·99) for influenza A IgA and 0·02 (95% CI 0·00–1·00) for influenza A PCR (Table 2). Both Bayesian LCA models yielded the same predicted group membership for influenza A (data not shown).

Influenza B

For influenza B a positive test result was observed in 244 subjects (25·7%) by influenza B IgG, in 57 subjects (6·0%) by influenza B IgA and in eight subjects (0·8%) by influenza B PCR (Table 1). In the estimated LCA model for influenza B a total of 29 subjects were classified as infected by both influenza B IgG and influenza B IgA (Supplementary Table S4). A very low sensitivity with 0·10 (95% CI 0·00–1·00) was estimated for influenza B PCR (Table 2). Influenza B IgG had a high false-positive rate resulting in a moderate specificity. Both Bayesian LCA models yielded the same predicted group membership for influenza B (data not shown).

DISCUSSION

In this cohort of adult patients in Germany who were coughing for ⩾7 days before seeking medical attention, the combination of serology and PCR seemed not only to improve the overall performance of diagnostic tests for B. pertussis but also for adenovirus, and influenza virus A and B infections.

For interpretation of our data some points of our study design are worth discussing: first, our inclusion criteria selected against detecting influenza-like illnesses, as the clinical definition of influenza would normally require an acute onset with high fever and pronounced malaise. In our study setting we found that patients were coughing for a median of 3 weeks before visiting a physician. Consequently, we assume that the detection of viral RNA for influenza virus A and B, as well as viral DNA for adenovirus may have a similarly low sensitivity as has been documented in adult pertussis cases for detection of Bordetella DNA [Reference von Konig2, Reference Riffelmann5]. In this respect, our study reproduced the assumption made in an earlier study using LCA [Reference Baughman3]. Our pre-analytics, however, may have additionally disadvantaged the detection of viral nucleic acids, as we used oropharyngeal washings that were found to be less sensitive than nasopharyngeal samples [Reference Lieberman21]. In that study, it was observed that in 550 hospitalized patients, viral RNA/DNA could be detected in 136 oropharyngeal swabs, and also in 184 nasopharyngeal swabs. However, at the time of our study, our protocol depended on oropharyngeal washings. Furthermore, the diagnostic gold standard is also a function of age. Whereas in adults, sensitivity of PCR is rather low, it can be around 70% in infants or young children who visit their physician/paediatrician early after the onset of cough [Reference Riffelmann5].

The specificity of the antigens used in diagnostic serology may be another reason for concern. In pertussis serology, recommendations about the use of specific antigens have been published [Reference Guiso9], but many serological kits still need to evolve and follow the consensus recommendations, which is not always the case. This is a major problem not only for routine biological diagnosis but also epidemiological studies. In influenza serology, and even less so in adenoviral serology, no consensus about antigens useful in the diagnosis of respiratory disease has been achieved. The commercial ELISA systems employed in this study used nucleoproteins for influenza A and B serology and hexon protein for adenovirus serology. For influenza serology these tests have been successfully used in diagnostic serology [Reference Voeten22] with a good sensitivity and specificity. For adenovirus respiratory infections in non-immunocompromised adults, isotype-specific ELISA systems were only rarely used [Reference Julkunen, Lehtomaki and Hovi23], but displayed sufficient sensitivity and specificity.

We deliberately did not confine the analyses to cases with confirmed coughing between 7 days and 3 months. Instead we chose an ‘intention to diagnose’ approach to be as close as possible to the physicians' diagnostic perspective. According to the physician, all patients had met the predefined case definition and for these patients the potential diagnostic properties of our test combination needed to be established.

The LCA model used here is a well-documented and statistically valid tool in the absence of a gold standard [Reference Baughman3, Reference Rutjes4] This approach has been used in another cohort with suspected pertussis [Reference Baughman3], but has not previously been applied to a combined set of tests for pertussis, adenovirus, and influenza A and B in a large population of adult patients with respiratory disease and cough. A methodological strength of our analysis is the validation of the frequentist approach by Bayesian approaches. A methodological limitation of this approach is that a combination of only three tests was applied. The total number of ‘true’ cases identified might be greater if a further set of diagnostic tests had been be available for the LCA. Due to the limited number of tests underlying the analysis, we could not use the random-effects model proposed by Qu et al. [Reference Qu, Tan and Kutner12] that integrate local dependence between tests through a single normally distributed random effect [Reference Reboussin, Ip and Wolfson24]. This may be a critical issue since the assumption of conditional independence is often violated in practice [Reference Rutjes4, Reference Qu, Tan and Kutner12, Reference Reboussin, Ip and Wolfson24, Reference Pepe and Janes25]. It has been shown that ignoring conditional independence biases the estimates of diagnostic accuracy. Even under study conditions, however, a combination of more than three tests is very unusual, and in clinical diagnostic practice diagnostic tests for outpatients with chronic coughs are rarely if ever applied. Thus, a recently published clinical guideline on acute coughs in adults [Reference Holzinger26] only mentions pertussis when a laboratory diagnosis may be attempted.

We partly estimated wide confidence limits for the sensitivity or specificity. This could be caused by no or only a few subjects in some response patterns, leading to a very flat likelihood. In this case, the estimates will have a high variance even if the likelihood is identifiable [Reference Madans27].

The role of acute infections in chronic cough in adults without underlying lung disease was unknown. In a population of >900 individuals with clinical signs of respiratory disease and cough and without positive PCR, additional cases of B. pertussis, adenovirus, and influenza virus A and B infections were identified by serology (Table 1). For all conditions a combination of IgG and IgA serological testing had the best test performance while PCR had little overall value in this setting. Although PCR is generally regarded as the diagnostic ‘gold standard’, our study shows that for this patient group the addition of diagnostic viral serology may be a valuable adjunct for laboratory diagnosis. Given the constraints of the study, however, additional work is needed to prospectively define the optimal use of PCR and diagnostic serology in longer lasting coughing disease in adults.

APPENDIX. KRESH Sentinel Physicians

Krefeld: Frau und Herr Dr. Rieger, Praxis Dr. Krausbauer und Frau Dr. Möhrke, Herr Dr. Dotzel, Herr Dr. Frackenpohl, Praxis Dr. Lüdemann und Herr Dr. Schultz, Herr Dr. Urban, Herr Dr. Urlbauer, Herr Dr. Baselt, Herr Dr. Ridderskamp, Praxis Dr. Hochbruck und Dr. Hermann, Praxis Dr. Kemmerich und Dr. Thomaßen, Herr Dr. Meißner, Herr Dr. Seelhoff.

Rostock: Frau Dr. Lusch, Herr Dr. Rothe, Frau Dr. Krüger, Herr Dr. Th. Hohlbein, Frau Dr. Borchmann, Frau Dr. Kähler, Frau Dr. Bichowski, Frau Dr. Lüder, Frau Dr. Glaser, Frau Dr. B. Hohlbein, Frau Dr. Vilbrandt, Herr Dr. Anft, Frau Dr. Burow, Frau Dr. Olwig, Frau Dr. Engelhardt, Frau Dr. Lange, Herr Dr. Langer, Frau Dr. Evert, Frau Dr. Michelsen, Frau Dr. Frank, Frau Dr. Morcan

SUPPLEMENTARY MATERIAL

For supplementary material accompanying this paper visit http://dx.doi.org/10.1017/S0950268815002149.

ACKNOWLEDGEMENTS

The recruiting of patients and the logistics in this study was funded jointly by GlaxoSmithKline Pharma GmbH & Co. KG, Munich, Germany and Sanofi Pasteur MSD GmbH, Leimen, Germany. No funding was received for the statistical evaluation of for performing various diagnostic tests.

DECLARATION OF INTEREST

None.

References

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Figure 0

Fig. 1. Age distribution of study patients.

Figure 1

Table 1. Overall test results for polymerase chain reaction (PCR) and serology

Figure 2

Table 2. Estimated sensitivity and specificity of indicators of pertussis, adenovirus and influenza according to latent class analysis

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