Evaluation of pneumococcal load in blood by polymerase chain reaction for the diagnosis of pneumococcal pneumonia in young children in the PERCH study

Maria Deloria Knoll; Susan C. Morpeth; J. Anthony G. Scott; Nora L. Watson; Daniel E. Park; Henry C. Baggett; W. Abdullah Brooks; Daniel R. Feikin; Laura L. Hammitt; Stephen R.C. Howie; Karen L. Kotloff; Orin S. Levine; Katherine L. O'Brien; Donald M. Thea; Dilruba Ahmed; Martin Antonio; Juliet O. Awori; Vicky L. Baillie; James Chipeta; Andrea N. Deluca; Michel Dione; Amanda J. Driscoll; Melissa M. Higdon; Anchalee Jatapai; Ruth A. Karron; Razib Mazumder; David P. Moore; James Mwansa; Sammy Nyongesa; Christine Prosperi; Phil Seidenberg; Duangkamon Siludjai; Samba O. Sow; Boubou Tamboura; Scott L. Zeger; David R. Murdoch; Shabir A. Madhi; Nicholas Fancourt; Wei Fu; E. Wangeci Kagucia; Mengying Li; Zhenke Wu; Jane Crawley; Hubert P. Endtz; Khalequ Zaman; Doli Goswami; Lokman Hossain; Yasmin Jahan; Hasan Ashraf; Alice Kamau

doi:10.1093/cid/cix149

Evaluation of pneumococcal load in blood by polymerase chain reaction for the diagnosis of pneumococcal pneumonia in young children in the PERCH study

Maria Deloria Knoll
, Susan C. Morpeth
, J. Anthony G. Scott
, Nora L. Watson
, Daniel E. Park
, Henry C. Baggett
, W. Abdullah Brooks
, Daniel R. Feikin
, Laura L. Hammitt
, Stephen R.C. Howie
, Karen L. Kotloff
, Orin S. Levine
, Katherine L. O'Brien
, Donald M. Thea
, Dilruba Ahmed
, Martin Antonio
, Juliet O. Awori
, Vicky L. Baillie
, James Chipeta
, Andrea N. Deluca

Michel Dione, Amanda J. Driscoll, Melissa M. Higdon, Anchalee Jatapai, Ruth A. Karron, Razib Mazumder, David P. Moore, James Mwansa, Sammy Nyongesa, Christine Prosperi, Phil Seidenberg, Duangkamon Siludjai, Samba O. Sow, Boubou Tamboura, Scott L. Zeger, David R. Murdoch, Shabir A. Madhi, Nicholas Fancourt, Wei Fu, E. Wangeci Kagucia, Mengying Li, Zhenke Wu, Jane Crawley, Hubert P. Endtz, Khalequ Zaman, Doli Goswami, Lokman Hossain, Yasmin Jahan, Hasan Ashraf, Alice Kamau

Johns Hopkins University
Kenya Medical Research Institute
London School of Hygiene and Tropical Medicine
Middlemore Hospital
The EMMES Corporation
George Washington University
Thailand Ministry of Public Health-US Centers for Disease Control and Prevention Collaboration
Centers for Disease Control and Prevention
International Centre for Diarrhoeal Disease Research Bangladesh
The University of Auckland
University of Otago
University of Maryland, Baltimore
Gates Foundation
Boston University
University of Warwick
University of the Witwatersrand
University of Zambia
International Livestock Research Institute
University Teaching Hospital Lusaka
Zambia Center for Applied Health Research and Development
University of New Mexico
Centre pour le Développement des Vaccines (CVD-Mali)
Canterbury District Health Board
University of Oxford

Research output: Contribution to journal › Article › peer-review

25 Citations (Scopus)

Abstract

Background. Detection of pneumococcus by lytA polymerase chain reaction (PCR) in blood had poor diagnostic accuracy for diagnosing pneumococcal pneumonia in children in 9 African and Asian sites. We assessed the value of blood lytA quantification in diagnosing pneumococcal pneumonia. Methods. The Pneumonia Etiology Research for Child Health (PERCH) case-control study tested whole blood by PCR for pneumococcus in children aged 1-59 months hospitalized with signs of pneumonia and in age-frequency matched community controls. The distribution of load among PCR-positive participants was compared between microbiologically confirmed pneumococcal pneumonia (MCPP) cases, cases confirmed for nonpneumococcal pathogens, nonconfirmed cases, and controls. Receiver operating characteristic analyses determined the "optimal threshold" that distinguished MCPP cases from controls. Results. Load was available for 290 of 291 cases with pneumococcal PCR detected in blood and 273 of 273 controls. Load was higher in MCPP cases than controls (median, 4.0 × 103 vs 0.19 × 103 copies/mL), but overlapped substantially (range, 0.16-989.9 × 103 copies/mL and 0.01-551.9 × 103 copies/mL, respectively). The proportion with high load (≥2.2 log10 copies/mL) was 62.5% among MCPP cases, 4.3% among nonconfirmed cases, 9.3% among cases confirmed for a nonpneumococcal pathogen, and 3.1% among controls. Pneumococcal load in blood was not associated with respiratory tract illness in controls (P = .32). High blood pneumococcal load was associated with alveolar consolidation on chest radiograph in nonconfirmed cases, and with high (>6.9 log10 copies/mL) nasopharyngeal/oropharyngeal load and C-reactive protein ≥40 mg/L (both P < .01) in nonconfirmed cases but not controls. Conclusions. Quantitative pneumococcal PCR in blood has limited diagnostic utility for identifying pneumococcal pneumonia in individual children, but may be informative in epidemiological studies.

Original language	English
Pages (from-to)	S357-S367
Journal	Clinical Infectious Diseases
Volume	64
DOIs	https://doi.org/10.1093/cid/cix149
Publication status	Published - 1 Jan 2017
Externally published	Yes

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

SDG 3 Good Health and Well-being

Keywords

Blood
Diagnosis
PCR
Pneumococcus
Pneumonia

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10.1093/cid/cix149Licence: CC BY

Cite this

Knoll, M. D., Morpeth, S. C., Scott, J. A. G., Watson, N. L., Park, D. E., Baggett, H. C., Brooks, W. A., Feikin, D. R., Hammitt, L. L., Howie, S. R. C., Kotloff, K. L., Levine, O. S., O'Brien, K. L., Thea, D. M., Ahmed, D., Antonio, M., Awori, J. O., Baillie, V. L., Chipeta, J., ... Kamau, A. (2017). Evaluation of pneumococcal load in blood by polymerase chain reaction for the diagnosis of pneumococcal pneumonia in young children in the PERCH study. Clinical Infectious Diseases, 64, S357-S367. https://doi.org/10.1093/cid/cix149

@article{fef18aab0299443080d05caf8658badd,

title = "Evaluation of pneumococcal load in blood by polymerase chain reaction for the diagnosis of pneumococcal pneumonia in young children in the PERCH study",

abstract = "Background. Detection of pneumococcus by lytA polymerase chain reaction (PCR) in blood had poor diagnostic accuracy for diagnosing pneumococcal pneumonia in children in 9 African and Asian sites. We assessed the value of blood lytA quantification in diagnosing pneumococcal pneumonia. Methods. The Pneumonia Etiology Research for Child Health (PERCH) case-control study tested whole blood by PCR for pneumococcus in children aged 1-59 months hospitalized with signs of pneumonia and in age-frequency matched community controls. The distribution of load among PCR-positive participants was compared between microbiologically confirmed pneumococcal pneumonia (MCPP) cases, cases confirmed for nonpneumococcal pathogens, nonconfirmed cases, and controls. Receiver operating characteristic analyses determined the {"}optimal threshold{"} that distinguished MCPP cases from controls. Results. Load was available for 290 of 291 cases with pneumococcal PCR detected in blood and 273 of 273 controls. Load was higher in MCPP cases than controls (median, 4.0 × 103 vs 0.19 × 103 copies/mL), but overlapped substantially (range, 0.16-989.9 × 103 copies/mL and 0.01-551.9 × 103 copies/mL, respectively). The proportion with high load (≥2.2 log10 copies/mL) was 62.5\% among MCPP cases, 4.3\% among nonconfirmed cases, 9.3\% among cases confirmed for a nonpneumococcal pathogen, and 3.1\% among controls. Pneumococcal load in blood was not associated with respiratory tract illness in controls (P = .32). High blood pneumococcal load was associated with alveolar consolidation on chest radiograph in nonconfirmed cases, and with high (>6.9 log10 copies/mL) nasopharyngeal/oropharyngeal load and C-reactive protein ≥40 mg/L (both P < .01) in nonconfirmed cases but not controls. Conclusions. Quantitative pneumococcal PCR in blood has limited diagnostic utility for identifying pneumococcal pneumonia in individual children, but may be informative in epidemiological studies.",

keywords = "Blood, Diagnosis, PCR, Pneumococcus, Pneumonia",

author = "Knoll, \{Maria Deloria\} and Morpeth, \{Susan C.\} and Scott, \{J. Anthony G.\} and Watson, \{Nora L.\} and Park, \{Daniel E.\} and Baggett, \{Henry C.\} and Brooks, \{W. Abdullah\} and Feikin, \{Daniel R.\} and Hammitt, \{Laura L.\} and Howie, \{Stephen R.C.\} and Kotloff, \{Karen L.\} and Levine, \{Orin S.\} and O'Brien, \{Katherine L.\} and Thea, \{Donald M.\} and Dilruba Ahmed and Martin Antonio and Awori, \{Juliet O.\} and Baillie, \{Vicky L.\} and James Chipeta and Deluca, \{Andrea N.\} and Michel Dione and Driscoll, \{Amanda J.\} and Higdon, \{Melissa M.\} and Anchalee Jatapai and Karron, \{Ruth A.\} and Razib Mazumder and Moore, \{David P.\} and James Mwansa and Sammy Nyongesa and Christine Prosperi and Phil Seidenberg and Duangkamon Siludjai and Sow, \{Samba O.\} and Boubou Tamboura and Zeger, \{Scott L.\} and Murdoch, \{David R.\} and Madhi, \{Shabir A.\} and Nicholas Fancourt and Wei Fu and Kagucia, \{E. Wangeci\} and Mengying Li and Zhenke Wu and Jane Crawley and Endtz, \{Hubert P.\} and Khalequ Zaman and Doli Goswami and Lokman Hossain and Yasmin Jahan and Hasan Ashraf and Alice Kamau",

year = "2017",

month = jan,

day = "1",

doi = "10.1093/cid/cix149",

language = "English",

volume = "64",

pages = "S357--S367",

journal = "Clinical Infectious Diseases",

issn = "1058-4838",

publisher = "Oxford University Press",

}

Knoll, MD, Morpeth, SC, Scott, JAG, Watson, NL, Park, DE, Baggett, HC, Brooks, WA, Feikin, DR, Hammitt, LL, Howie, SRC, Kotloff, KL, Levine, OS, O'Brien, KL, Thea, DM, Ahmed, D, Antonio, M, Awori, JO, Baillie, VL, Chipeta, J, Deluca, AN, Dione, M, Driscoll, AJ, Higdon, MM, Jatapai, A, Karron, RA, Mazumder, R, Moore, DP, Mwansa, J, Nyongesa, S, Prosperi, C, Seidenberg, P, Siludjai, D, Sow, SO, Tamboura, B, Zeger, SL, Murdoch, DR, Madhi, SA, Fancourt, N, Fu, W, Kagucia, EW, Li, M, Wu, Z, Crawley, J, Endtz, HP, Zaman, K, Goswami, D, Hossain, L, Jahan, Y, Ashraf, H & Kamau, A 2017, 'Evaluation of pneumococcal load in blood by polymerase chain reaction for the diagnosis of pneumococcal pneumonia in young children in the PERCH study', Clinical Infectious Diseases, vol. 64, pp. S357-S367. https://doi.org/10.1093/cid/cix149

TY - JOUR

T1 - Evaluation of pneumococcal load in blood by polymerase chain reaction for the diagnosis of pneumococcal pneumonia in young children in the PERCH study

AU - Knoll, Maria Deloria

AU - Morpeth, Susan C.

AU - Scott, J. Anthony G.

AU - Watson, Nora L.

AU - Park, Daniel E.

AU - Baggett, Henry C.

AU - Brooks, W. Abdullah

AU - Feikin, Daniel R.

AU - Hammitt, Laura L.

AU - Howie, Stephen R.C.

AU - Kotloff, Karen L.

AU - Levine, Orin S.

AU - O'Brien, Katherine L.

AU - Thea, Donald M.

AU - Ahmed, Dilruba

AU - Antonio, Martin

AU - Awori, Juliet O.

AU - Baillie, Vicky L.

AU - Chipeta, James

AU - Deluca, Andrea N.

AU - Dione, Michel

AU - Driscoll, Amanda J.

AU - Higdon, Melissa M.

AU - Jatapai, Anchalee

AU - Karron, Ruth A.

AU - Mazumder, Razib

AU - Moore, David P.

AU - Mwansa, James

AU - Nyongesa, Sammy

AU - Prosperi, Christine

AU - Seidenberg, Phil

AU - Siludjai, Duangkamon

AU - Sow, Samba O.

AU - Tamboura, Boubou

AU - Zeger, Scott L.

AU - Murdoch, David R.

AU - Madhi, Shabir A.

AU - Fancourt, Nicholas

AU - Fu, Wei

AU - Kagucia, E. Wangeci

AU - Li, Mengying

AU - Wu, Zhenke

AU - Crawley, Jane

AU - Endtz, Hubert P.

AU - Zaman, Khalequ

AU - Goswami, Doli

AU - Hossain, Lokman

AU - Jahan, Yasmin

AU - Ashraf, Hasan

AU - Kamau, Alice

PY - 2017/1/1

Y1 - 2017/1/1

N2 - Background. Detection of pneumococcus by lytA polymerase chain reaction (PCR) in blood had poor diagnostic accuracy for diagnosing pneumococcal pneumonia in children in 9 African and Asian sites. We assessed the value of blood lytA quantification in diagnosing pneumococcal pneumonia. Methods. The Pneumonia Etiology Research for Child Health (PERCH) case-control study tested whole blood by PCR for pneumococcus in children aged 1-59 months hospitalized with signs of pneumonia and in age-frequency matched community controls. The distribution of load among PCR-positive participants was compared between microbiologically confirmed pneumococcal pneumonia (MCPP) cases, cases confirmed for nonpneumococcal pathogens, nonconfirmed cases, and controls. Receiver operating characteristic analyses determined the "optimal threshold" that distinguished MCPP cases from controls. Results. Load was available for 290 of 291 cases with pneumococcal PCR detected in blood and 273 of 273 controls. Load was higher in MCPP cases than controls (median, 4.0 × 103 vs 0.19 × 103 copies/mL), but overlapped substantially (range, 0.16-989.9 × 103 copies/mL and 0.01-551.9 × 103 copies/mL, respectively). The proportion with high load (≥2.2 log10 copies/mL) was 62.5% among MCPP cases, 4.3% among nonconfirmed cases, 9.3% among cases confirmed for a nonpneumococcal pathogen, and 3.1% among controls. Pneumococcal load in blood was not associated with respiratory tract illness in controls (P = .32). High blood pneumococcal load was associated with alveolar consolidation on chest radiograph in nonconfirmed cases, and with high (>6.9 log10 copies/mL) nasopharyngeal/oropharyngeal load and C-reactive protein ≥40 mg/L (both P < .01) in nonconfirmed cases but not controls. Conclusions. Quantitative pneumococcal PCR in blood has limited diagnostic utility for identifying pneumococcal pneumonia in individual children, but may be informative in epidemiological studies.

AB - Background. Detection of pneumococcus by lytA polymerase chain reaction (PCR) in blood had poor diagnostic accuracy for diagnosing pneumococcal pneumonia in children in 9 African and Asian sites. We assessed the value of blood lytA quantification in diagnosing pneumococcal pneumonia. Methods. The Pneumonia Etiology Research for Child Health (PERCH) case-control study tested whole blood by PCR for pneumococcus in children aged 1-59 months hospitalized with signs of pneumonia and in age-frequency matched community controls. The distribution of load among PCR-positive participants was compared between microbiologically confirmed pneumococcal pneumonia (MCPP) cases, cases confirmed for nonpneumococcal pathogens, nonconfirmed cases, and controls. Receiver operating characteristic analyses determined the "optimal threshold" that distinguished MCPP cases from controls. Results. Load was available for 290 of 291 cases with pneumococcal PCR detected in blood and 273 of 273 controls. Load was higher in MCPP cases than controls (median, 4.0 × 103 vs 0.19 × 103 copies/mL), but overlapped substantially (range, 0.16-989.9 × 103 copies/mL and 0.01-551.9 × 103 copies/mL, respectively). The proportion with high load (≥2.2 log10 copies/mL) was 62.5% among MCPP cases, 4.3% among nonconfirmed cases, 9.3% among cases confirmed for a nonpneumococcal pathogen, and 3.1% among controls. Pneumococcal load in blood was not associated with respiratory tract illness in controls (P = .32). High blood pneumococcal load was associated with alveolar consolidation on chest radiograph in nonconfirmed cases, and with high (>6.9 log10 copies/mL) nasopharyngeal/oropharyngeal load and C-reactive protein ≥40 mg/L (both P < .01) in nonconfirmed cases but not controls. Conclusions. Quantitative pneumococcal PCR in blood has limited diagnostic utility for identifying pneumococcal pneumonia in individual children, but may be informative in epidemiological studies.

KW - Blood

KW - Diagnosis

KW - PCR

KW - Pneumococcus

KW - Pneumonia

U2 - 10.1093/cid/cix149

DO - 10.1093/cid/cix149

M3 - Article

SN - 1058-4838

VL - 64

SP - S357-S367

JO - Clinical Infectious Diseases

JF - Clinical Infectious Diseases

ER -

Evaluation of pneumococcal load in blood by polymerase chain reaction for the diagnosis of pneumococcal pneumonia in young children in the PERCH study

Abstract

UN SDGs

Keywords

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