Etiologic Diagnosis of Adult Bacterial Pneumonia by Culture and PCR Applied to Respiratory Tract Samples

Strålin, Kristoffer; Tornqvist, Ewa Wigaeus; Kaltoft, Margit S.; Olcén, Per; Holmberg, Hans

doi:10.1128/jcm.44.2.643-645.2006

Cited by 75 publications

(52 citation statements)

References 16 publications

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“…PCR has previously been shown to identify a high rate of colonisation of H. influenzae in patients with chronic obstructive pulmonary disease [33], but H. influenzae was also identified in 22% by BAL culture and 37% by BAL mPCR in 27 patients who had never smoked. As mPCR has shown a high analytical specificity for H. influenzae [12], and as sputum mPCR was positive for H. influenzae in only two (7.7%) out of 26 CAP patients with definite aetiologies other than H. influenzae in the present authors' previous study [13], the high rate of H. influenzae in the present study probably represents colonisation. Hence, it would be interesting to test mPCR on BAL samples from another LRTI population and another control population with a lower smoking frequency.…”

Section: Discussionsupporting

confidence: 51%

“…In the present authors' previous study of 235 patients with CAP [13], three patients were microimmunofluorescence-test positive for C. pneumoniae in paired sera; these three patients were also mPCR positive for C. pneumoniae in nasopharyngeal secretions. The fact that no control and only one LRTI patient was BAL mPCR positive in the present study indicates that BAL mPCR is probably specific for C. pneumoniae.…”

Section: Discussionmentioning

confidence: 50%

“…The method showed an analytical sensitivity of 100% (89 out of 89) and a specificity of 99% (167 out of 168) when 257 bacterial strains (37 different species) were tested [12]. mPCR has been evaluated on sputum samples and nasopharyngeal samples from adults with community-acquired pneumonia (CAP) and controls with promising results [13].…”

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confidence: 99%

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Evaluation of a multiplex PCR for bacterial pathogens applied to bronchoalveolar lavage

Strålin

Korsgaard²,

Olcén³

2006

European Respiratory Journal

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The present study assessed the diagnostic usefulness of a multiplex PCR (mPCR) for Streptococcus pneumoniae, Haemophilus influenzae, Mycoplasma pneumoniae and Chlamydophila pneumoniae applied to bronchoalveolar lavage (BAL).Fibreoptic bronchoscopy was performed on 156 hospitalised adult patients with lower respiratory tract infection (LRTI) and 36 controls. BAL fluid was analysed with bacterial culture and mPCR.By conventional diagnostic methods, S. pneumoniae, H. influenzae, M. pneumoniae and C. pneumoniae were aetiological agents in 14, 21, 3.2 and 0% of the LRTI patients, respectively. These pathogens were identified by BAL mPCR in 28, 47, 3.2 and 0.6% of cases, respectively, yielding sensitivities of 86% for S. pneumoniae, 88% for H. influenzae, 100% for M. pneumoniae and 0% for C. pneumoniae, and specificities of 81, 64, 100 and 99% for S. pneumoniae, H. influenzae, M. pneumoniae and C. pneumoniae, respectively. Of the 103 patients who had taken antibiotics prior to bronchoscopy, S. pneumoniae was identified by culture in 2.9% and by mPCR in 31%. Among the controls, mPCR identified S. pneumoniae in 11% and H. influenzae in 39%.In lower respiratory tract infection patients, bronchoalveolar lavage multiplex PCR can be useful for identification of Streptococcus pneumoniae, Mycoplasma pneumoniae and Chlamydophila pneumoniae. The method appears to be particularly useful in patients treated with antibiotics.

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Section: Discussionsupporting

confidence: 51%

Section: Discussionmentioning

confidence: 50%

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Evaluation of a multiplex PCR for bacterial pathogens applied to bronchoalveolar lavage

Strålin

Korsgaard²,

Olcén³

2006

European Respiratory Journal

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“…The sensitivity of plyNCR PCR for the detection of pneumococcal colonization was significantly higher than that of conventional culture (50% versus 40%). This corresponds to the results for other PCR-based methods for the detection of pneumococcal colonization directly in nasopharyngeal swabs (15,28).…”

Section: Discussionsupporting

confidence: 81%

Detection of Streptococcus pneumoniae Strain Cocolonization in the Nasopharynx

2009

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Colonization with more than one distinct strain of the same species, also termed cocolonization, is a prerequisite for horizontal gene transfer between pneumococcal strains that may lead to change of the capsular serotype. Capsule switch has become an important issue since the introduction of conjugated pneumococcal polysaccharide vaccines. There is, however, a lack of techniques to detect multiple colonization by S. pneumoniae strains directly in nasopharyngeal samples. Two hundred eighty-seven nasopharyngeal swabs collected during the prevaccine era within a nationwide surveillance program were analyzed by a novel technique for the detection of cocolonization, based on PCR amplification of a noncoding region adjacent to the pneumolysin gene (plyNCR) and restriction fragment length polymorphism (RFLP) analysis. The numbers of strains and their relative abundance in cocolonized samples were determined by terminal RFLP. The pneumococcal carriage rate found by PCR was 51.6%, compared to 40.0% found by culture. Cocolonization was present in 9.5% (10/105) of samples, most (9/10) of which contained two strains in a ratio of between 1:1 and 17:1. Five of the 10 cocolonized samples showed combinations of vaccine types only (n ‫؍‬ 2) or combinations of nonvaccine types only (n ‫؍‬ 3). Carriers of multiple pneumococcal strains had received recent antibiotic treatment more often than those colonized with a single strain (33% versus 9%, P ‫؍‬ 0.025). This new technique allows for the rapid and economical study of pneumococcal cocolonization in nasopharyngeal swabs. It will be valuable for the surveillance of S. pneumoniae epidemiology under vaccine selection pressure.Streptococcus pneumoniae is among the most important of human pathogens and is responsible for bacterial meningitis, sepsis, pneumonia, and acute otitis media. The habitat of the pneumococcus is the mucosa of the human nasopharynx. Colonization of the nasopharynx occurs early in life, with a prevalence of about 40% in infants and 15% in adults (depending on the local epidemiology). A single strain can persist in the nasopharynx for weeks or months, to then be replaced by other strains. Colonization is the starting point for all relevant aspects of this pathogen, such as invasive disease, exchange of genetic material, genetic recombination, and transmission. By the age of two, more than 95% of children have been colonized with up to six different serotypes (8). Sometimes more than one pneumococcal strain colonizes the nasopharynx at the same time. This phenomenon is known as cocolonization, or multiple colonization with more than one distinct strain of the same species. Cocolonization is probably required for horizontal gene transfer between different pneumococcal strains. Such genetic exchange has been shown to occur for the capsule gene locus and has been observed in the past for dominant international multiresistant pneumococcal clones (5). There are few data on rates of multiple colonization, but existing estimates range from 1.3% (13) up to 20% (9, 26). No...

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“…In general, when performed on sputum samples they have good sensitivity but poor specificity (12,17). In order to overcome the latter problem, PCR assays have been evaluated on blood samples (5,8,14,15), giving excellent specificity but relatively poor sensitivity.…”

mentioning

confidence: 99%

Diagnosis of Streptococcus pneumoniae Infections in Adults with Bacteremia and Community-Acquired Pneumonia: Clinical Comparison of Pneumococcal PCR and Urinary Antigen Detection

Smith

Sheppard²,

Hogan

et al. 2009

J Clin Microbiol

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The diagnosis of severe Streptococcus pneumoniae infection relies heavily on insensitive culture techniques. To improve the usefulness of PCR assays, we developed a dual-PCR protocol (targeted at pneumolysin and autolysin) for EDTA blood samples. This was compared to the Binax NOW S. pneumoniae urine antigen test in patients with bacteremic pneumococcal infections. Patients with nonbacteremic community-acquired pneumonia also were tested by these methods to determine what proportion could be confirmed as pneumococcal infections. A direct comparison was made in a group of patients who each had both tests performed. The Binax NOW S. pneumoniae urine antigen test was positive in 51 of 58 bacteremic pneumococcal cases (sensitivity, 88%; 95% confidence interval [CI], 77 to 95%), whereas the dual PCR was positive in 31 cases (sensitivity, 53.5%; 95% CI, 40 to 67%; P < 0.0001), and all of these had detectable urinary antigens. Both tests gave positive results in 2 of 51 control patients (referred to as other-organism septicemia), giving a specificity of 96% (95% CI, 86.5 to 99.5%). In 77 patients with nonbacteremic community-acquired pneumonia, urinary antigen was detected significantly more often (in 21 patients [27%]) than a positive result by the dual-PCR protocol (6 [8%]) (P ‫؍‬ 0.002). The development of a dual-PCR protocol enhanced the sensitivity compared to that of the individual assays, but it is still significantly less sensitive than the Binax NOW urine antigen test, as well as being more time-consuming and expensive. Urinary antigen detection is the nonculture diagnostic method of choice for patients with possible severe pneumococcal infection.

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Etiologic Diagnosis of Adult Bacterial Pneumonia by Culture and PCR Applied to Respiratory Tract Samples

Cited by 75 publications

References 16 publications

Evaluation of a multiplex PCR for bacterial pathogens applied to bronchoalveolar lavage

Evaluation of a multiplex PCR for bacterial pathogens applied to bronchoalveolar lavage

Detection of Streptococcus pneumoniae Strain Cocolonization in the Nasopharynx

Diagnosis of Streptococcus pneumoniae Infections in Adults with Bacteremia and Community-Acquired Pneumonia: Clinical Comparison of Pneumococcal PCR and Urinary Antigen Detection

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