S K Skelton scite author profile

Avian chlamydiosis was detected in a shipment of ú700 pet birds from a Florida bird distributor that were sold to nine Atlanta-area pet stores in August 1995. Respiratory illness among persons who had recently acquired birds from this shipment was reported to local public health officials. The attack rate of acute respiratory illness was 10.7% among persons in households exposed to birds from the implicated flock vs. 1.8% among control households (odds ratio, 6.60; 95% confidence interval, 1.39 -31.2). Illness and serological evidence of infection in the absence of symptoms were more common among persons in households with recently purchased birds that were sick or that had died and among persons who had had direct contact with the birds. Clinical psittacosis or serological evidence of Chlamydia psittaci infection was found in 30.7% of households with birds from the infected flock. Mild illnesses and asymptomatic infections in exposed persons were unusual features of this outbreak.

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Application of a nested, multiplex PCR to psittacosis outbreaks

Messmer

et al. 1997

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We developed a nested, multiplex PCR for simultaneous detection of three species of chlamydiae in human and avian specimens. The PCR was designed to increase sensitivity and to circumvent inhibitors of PCR present in clinical specimens. The target sequence was the 16S rRNA gene. The first-step PCR was genus specific, and the second-step PCR was multiplexed (i.e., had multiple primer sets in the same tube) and could discriminate among Chlamydia pneumoniae, Chlamydia psittaci, and Chlamydia trachomatis on the basis of the molecular weight of the amplicon. The limit of detection of each of the two PCR steps was 5 inclusion-forming units. We used PCR and serologic evidence during outbreaks of psittacosis to infer that C. psittaci had been transmitted from birds purchased in pet stores to humans. We also used this method to test both live and dead birds from pet stores for infection with C. psittaci. Compared with culture, the application of PCR to avian specimens increased the rate of C. psittaci detection.

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Efficient culture of Chlamydia pneumoniae with cell lines derived from the human respiratory tract

1992

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Two established cell lines, H 292 and HEp-2, originating from the human respiratory tract, were found to be significantly more efficient and practical than the currently used HeLa 229 cells for growth of Chlamydia pneumoniae. Six strains of C. pneunoniae recently isolated from patients with respiratory ailments were used as test cultures. The H 292 and HEp-2 cells yielded much higher inclusion counts for all the test strains than did HeLa 229 cells. When they were compared with each other, H 292 cells yielded more inclusions than did HEp-2 cells, and the differences were statistically significant in 10 of 18 test sets. A simple system with these two cell lines appeared to be very efficient for culturing C. pneumoniae. It does not require treatment of tissue cells with DEAE-dextran before infection, and it may eliminate the need for serial subpassages of specimens to increase culture sensitivity. Monolayers of these cells remained intact and viable in the Chlamydia growth medium so that reinfection could take place, resulting in greatly increased inclusion counts for specimens containing few infectious units. This system may make it more practical for laboratories to culture for C. pneumoniae for treatment of infections and outbreak intervention and will facilitate studies on this recently recognized pathogen. * Corresponding author. were isolated from patients with respiratory ailments in a military training camp in Norway during an adenovirus outbreak (1) and were kindly provided by Bjorn P. Berdal, University of Tromso, Tromso, Norway. All strains were isolated in HeLa 229 cells. Strain CWL 029 was used as antigen for production of monoclonal antibodies for identification of C. pneumoniae in tissue cells. The other six isolates in the third to fifth subpassages in HeLa 229 cells were used as inocula to test the selected cell lines. Serotype strains of C. trachomatis, originally from S. P. Wang of the University of Washington, Seattle, and C. psittaci PI-1 and D44 were from our stock cultures. Cell lines. All cell lines were obtained from the Cell Culture Section at the Centers for Disease Control and were passaged by standard tissue culture techniques. The following five cell lines derived from human respiratory tissues were tested in reference to HeLa 229 from cervix carcinoma:

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Radiographic appearance of Chlamydia pneumoniae (TWAR strain) respiratory infections. CBPIS Study Group. Community-based Pneumonia Incidence Study.

McConnell¹,

Plouffe²,

File³

et al. 1994

Radiology

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S K Skelton

Detection of Chlamydiosis in a Shipment of Pet Birds, Leading to Recognition of an Outbreak of Clinically Mild Psittacosis in Humans

Application of a nested, multiplex PCR to psittacosis outbreaks

Efficient culture of Chlamydia pneumoniae with cell lines derived from the human respiratory tract

Radiographic appearance of Chlamydia pneumoniae (TWAR strain) respiratory infections. CBPIS Study Group. Community-based Pneumonia Incidence Study.

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