A Sensitive, Specific, and Cost-Effective Multiplex Reverse Transcriptase-PCR Assay for the Detection of Seven Common Respiratory Viruses in Respiratory Samples

Syrmis, Melanie W.; Whiley, David M.; Thomas, Marion; Mackay, Ian M.; Williamson, Jeanette; Siebert, David; Nissen, Michael D.; Sloots, Theo P.

doi:10.1016/s1525-1578(10)60500-4

Cited by 159 publications

(172 citation statements)

References 36 publications

Supporting

Mentioning

153

Contrasting

Unclassified

Order By: Relevance

“…Hücre kültürü ve direkt immünofloresans yöntemleri, solunum yolu viral enfeksiyonlarının tanısında yaygınlıkla kullanılan geleneksel yöntemler olmakla birlikte, bu metotların duyarlılık ve özgüllüklerinde önemli kısıtlamalar bulunmaktadır 9 . Buna karşın, tek bir örnekten DNA ve RNA viruslarının tespitinde multipleks RT-PCR yöntemi duyarlı, özgül ve hızlı bir metottur 8 .…”

Section: Mi̇krobi̇yoloji̇ Bülteni̇unclassified

“…Günümüzde polimeraz zincir reaksiyonu (PCR) temelli testler, solunum yolu viruslarının tanımlanmasında, konvansiyonel yöntemlerden (virus izolasyonu ve antijen testleri) daha hızlı ve duyarlı sonuç vermektedir [6][7][8] . Özellikle çok sayıdaki solunum virusunu tek bir örnekte aynı anda tespit edebilen multipleks PCR/mikroarray yöntemlerinin kullanıma girmesi, gerek viral koenfeksiyonların prevalansının belirlenmesinde, gerekse doğru ve etkili antiviral tedaviye karar verilmesinde büyük yarar sağlamıştır 4,[8][9][10] .…”

Section: Introductionunclassified

See 1 more Smart Citation

Determination of the Frequency of Human Bocavirus and Other Respiratory Viruses Among 0-2 Years Age Group Children Diagnosed as Acute Bronchiolitis

Uyar¹,

Kuyucu²,

Tezcan³

et al. 2014

Mikrobiyol Bul

View full text Add to dashboard Cite

* Bu çalışma, Mersin Üniversitesi Bilimsel Araştırma Projeleri Birimi tarafından desteklenmiştir (Proje no. TF DTB [MU] 2010-4 TU). ÖZETAkut bronşiyolit, daha çok iki yaşından küçük çocuklarda sıklıkla viral etkenlerin neden olduğu bir alt solunum yolu enfeksiyonudur. Bu çalışmada, 0-2 yaş arası akut bronşiyolitli çocuklarda, insan bokavirusu (HBoV) da dahil olmak üzere solunum yolu viruslarının sıklığının belirlenmesi ve bu etkenlerle oluşan enfeksiyonların klinik özelliklerinin değerlendirilmesi amaçlanmıştır. Çalışmaya, Ocak-Haziran 2010 tarihleri arasında Mersin Üniversitesi Tıp Fakültesi, Çocuk Sağlığı ve Hastalıkları Anabilim Dalında akut bronşiyolit tanısı alan 62 hasta (45 erkek, 17 kız; yaş aralığı: 0-2 yıl) ile kontrol grubu olarak sağlıklı 33 çocuk (21 erkek, 12 kız; yaş aralığı: 0-2 yıl) dahil edilmiştir. Çalışma gruplarından alınan nazofarengeal aspirat örneklerinde solunum yolu virusları [respiratuar sinsityal virusu (RSV) A ve B; rhinovirus (RV); insan metapnömovirusu (hMPV) A ve B; influenza virus tip A (H1N1, H3N2, H1N1v), B ve C; parainfluenza virus (PIV) tip 1, 2, 3 ve 4A/B; adenovirus (AdV); HBoV; koronavirus (CoV 229E); enterovirus (EV)], multipleks polimeraz zincir reaksiyonu (M-PCR) ve DNA mikroarray prensibi ile çalışan CLART ® Pneumovir (Clinical Array Technology, Genomica, İspanya) ticari sistemi ile araştırılmıştır. Ayrıca, viral etkenler ile hastaların demografik, klinik ve laboratuvar özellikleri, uygulanan tedaviler ve hastanede yatış oranları arasındaki ilişki değerlendirilmiştir. Çalışmamızda, akut bronşiyolitli 62 hastanın 52 (%83.9)'sinde en az Geliş Tarihi (Received): 12.12.2013 • Kabul Ediliş Tarihi (Accepted): 11.04.2014

show abstract

Section: Mi̇krobi̇yoloji̇ Bülteni̇unclassified

Section: Introductionunclassified

Determination of the Frequency of Human Bocavirus and Other Respiratory Viruses Among 0-2 Years Age Group Children Diagnosed as Acute Bronchiolitis

Uyar¹,

Kuyucu²,

Tezcan³

et al. 2014

Mikrobiyol Bul

View full text Add to dashboard Cite

show abstract

“…We performed total cell and differential cell counts and identified bacterial, fungal, and mycobacterial pathogens from 500 L of BALF by standard methods reported elsewhere (16,17 ). We conducted direct immunofluorescence antigen testing for respiratory viruses on BALF as described (16 ); if results were negative, we performed nucleic acid amplification tests using a multiplex reverse transcriptase-PCR assay (18 ). Final counts for bacterial and fungal pathogens were expressed as CFU per mL of BALF.…”

Section: Balf Analysismentioning

confidence: 99%

Novel Neutrophil-Derived Proteins in Bronchoalveolar Lavage Fluid Indicate an Exaggerated Inflammatory Response in Pediatric Cystic Fibrosis Patients

et al. 2007

View full text Add to dashboard Cite

Background: Airway inflammation in cystic fibrosis (CF) is exaggerated and characterized by neutrophil-mediated tissue destruction, but its genesis and mechanisms remain poorly understood. To further define the pulmonary inflammatory response, we conducted a proteome-based screen of bronchoalveolar lavage fluid (BALF) collected from young children with and without CF experiencing endobronchial infection. Methods: We collected BALF samples from 45 children younger than 5 years and grouped them according to the presence of respiratory pathogens: ≥1 × 105 colony-forming units (CFU)/mL BALF (18 and 12 samples with and without CF, respectively) and <1 × 105 CFU/mL (23 and 15 samples). BALF proteins were analyzed with SELDI-TOF mass spectrometry (MS) and H4 ProteinChips®. Proteins were identified and characterized using trypsin digestion, tandem MS, Fourier transform ion cyclotron resonance MS, immunoblotting, and ELISA. Results: The SELDI-TOF MS BALF profiles contained 53 unique, reliably detected proteins. Peak intensities of 24 proteins differed significantly between the CF and non-CF samples. They included the neutrophil proteins, α-defensin 1 and 2, S100A8, S100A9, and S100A12, as well as novel forms of S100A8 and S100A12 with equivalent C-terminal deletions. Peak intensities of these neutrophil proteins and immunoreactive concentrations of selected examples were significantly higher in CF than non-CF samples. Conclusions: Small neutrophil-derived BALF proteins, including novel C-terminal truncated forms of S100A proteins, are easily detected with SELDI-TOF MS. Concentrations of these molecules are abnormally high in early CF lung disease. The data provide new insights into CF lung disease and identify novel proteins strongly associated with CF airway inflammation.

show abstract

“…The major surface glycoproteins, hemagglutinin (HA) and neuraminidase (NA), are primarily responsible for the antigenic variation seen in influenza viruses and serve as the basis for further subtyping of influenza type A viruses (51). The extreme genetic variability of influenza A viruses makes designing useful, rapid, molecular-based assays challenging (45), but several different approaches have been successfully utilized by targeting the highly conserved RNA gene segment encoding the internally expressed matrix 1 (M1) or nonstructural (NS) protein (16,44). Reverse transcription-PCR (RT-PCR) is effective for initial influenza diagnosis and has greater sensitivity than other available rapid assays (4,5,7,17,36).…”

mentioning

confidence: 99%

Evaluation of PCR Testing of Ethanol-Fixed Nasal Swab Specimens as an Augmented Surveillance Strategy for Influenza Virus and Adenovirus Identification

et al. 2005

View full text Add to dashboard Cite

Viral culture isolation has been widely accepted as the "gold standard" for laboratory confirmation of viral infection; however, it requires ultralow temperature specimen storage. Storage of specimens in ethanol at room temperature could expand our ability to conduct active surveillance and retrospective screenings of viruses with rapid and inexpensive real-time PCR tests, including isolates from remote regions where freezing specimens for culture is not feasible. Molecular methods allow for rapid identification of viral pathogens without the need to maintain viability. We hypothesized that ethanol, while inactivating viruses, can preserve DNA and RNA for PCR-based methods. To evaluate the use of ethanol-stored specimens for augmenting surveillance for detection of influenza viruses A and B and adenoviruses (AdV), paired nasal swab specimens were collected from 384 recruits with febrile respiratory illness at Fort Jackson, S.C., in a 2-year study. One swab was stored at ambient temperature in 100% ethanol for up to 6 months, and the other swab was stored at ؊70°C in viral medium. For viral detection, frozen specimens were cultured for a variety of respiratory viruses, and ethanol-fixed specimens were tested with TaqMan (TM) probe and LightCycler SYBR green (SG) melting curve assays with at least two different PCR targets for each virus. The sensitivities of the TM and SG assays on specimens stored in ethanol for 1 month were 75% and 58% for influenza A, 89% and 67% for influenza B, and 93 to 98% and 57% for AdV, respectively. Lower specificities of the real-time assays corresponded to the increased detection of PCR-positive but culture-negative specimens. Influenza virus RNA was detected as well or better after 6 months of storage in ethanol.

show abstract

A Sensitive, Specific, and Cost-Effective Multiplex Reverse Transcriptase-PCR Assay for the Detection of Seven Common Respiratory Viruses in Respiratory Samples

Cited by 159 publications

References 36 publications

Determination of the Frequency of Human Bocavirus and Other Respiratory Viruses Among 0-2 Years Age Group Children Diagnosed as Acute Bronchiolitis

Determination of the Frequency of Human Bocavirus and Other Respiratory Viruses Among 0-2 Years Age Group Children Diagnosed as Acute Bronchiolitis

Novel Neutrophil-Derived Proteins in Bronchoalveolar Lavage Fluid Indicate an Exaggerated Inflammatory Response in Pediatric Cystic Fibrosis Patients

Evaluation of PCR Testing of Ethanol-Fixed Nasal Swab Specimens as an Augmented Surveillance Strategy for Influenza Virus and Adenovirus Identification

Contact Info

Product

Resources

About