Detection of pneumococcal DNA in blood by polymerase chain reaction for diagnosing pneumococcal pneumonia in young children from low- and middle-income countries

Susan C. Morpeth; Maria Deloria Knoll; J. Anthony G. Scott; Daniel E. Park; Nora L. Watson; Henry C. Baggett; W. Abdullah Brooks; Daniel R. Feikin; Laura L. Hammitt; Stephen R.C. Howie; Karen L. Kotloff; Orin S. Levine; Shabir A. Madhi; Katherine L. O'Brien; Donald M. Thea; Peter V. Adrian; Dilruba Ahmed; Martin Antonio; Charatdao Bunthi; Andrea N. DeLuca; Amanda J. Driscoll; Louis Peter Githua; Melissa M. Higdon; Geoff Kahn; Angela Karani; Ruth A. Karron; Geoffrey Kwenda; Sirirat Makprasert; Razib Mazumder; David P. Moore; James Mwansa; Sammy Nyongesa; Christine Prosperi; Samba O. Sow; Boubou Tamboura; Toni Whistler; Scott L. Zeger; David R. Murdoch; Nicholas Fancourt; Wei Fu; E. Wangeci Kagucia; Mengying Li; Zhenke Wu; Jane Crawley; Hubert P. Endtz; Khalequ Zaman; Doli Goswami; Lokman Hossain; Yasmin Jahan; Alice Kamau

doi:10.1093/cid/cix145

Detection of pneumococcal DNA in blood by polymerase chain reaction for diagnosing pneumococcal pneumonia in young children from low- and middle-income countries

Susan C. Morpeth, Maria Deloria Knoll, J. Anthony G. Scott, Daniel E. Park, Nora L. Watson, Henry C. Baggett, W. Abdullah Brooks, Daniel R. Feikin, Laura L. Hammitt, Stephen R.C. Howie, Karen L. Kotloff, Orin S. Levine, Shabir A. Madhi, Katherine L. O'Brien, Donald M. Thea, Peter V. Adrian, Dilruba Ahmed, Martin Antonio, Charatdao Bunthi, Andrea N. DeLucaAmanda J. Driscoll, Louis Peter Githua, Melissa M. Higdon, Geoff Kahn, Angela Karani, Ruth A. Karron, Geoffrey Kwenda, Sirirat Makprasert, Razib Mazumder, David P. Moore, James Mwansa, Sammy Nyongesa, Christine Prosperi, Samba O. Sow, Boubou Tamboura, Toni Whistler, Scott L. Zeger, David R. Murdoch, Nicholas Fancourt, Wei Fu, E. Wangeci Kagucia, Mengying Li, Zhenke Wu, Jane Crawley, Hubert P. Endtz, Khalequ Zaman, Doli Goswami, Lokman Hossain, Yasmin Jahan, Alice Kamau

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

36 Citations (Scopus)

Abstract

Background. We investigated the performance of polymerase chain reaction (PCR) on blood in the diagnosis of pneumococcal pneumonia among children from 7 low- and middle-income countries. Methods. We tested blood by PCR for the pneumococcal autolysin gene in children aged 1-59 months in the Pneumonia Etiology Research for Child Health (PERCH) study. Children had World Health Organization-defined severe or very severe pneumonia or were age-frequency-matched community controls. Additionally, we tested blood from general pediatric admissions in Kilifi, Kenya, a PERCH site. The proportion PCR-positive was compared among cases with microbiologically confirmed pneumococcal pneumonia (MCPP), cases without a confirmed bacterial infection (nonconfirmed), cases confirmed for nonpneumococcal bacteria, and controls. Results. In PERCH, 7.3% (n = 291/3995) of cases and 5.5% (n = 273/4987) of controls were blood pneumococcal PCR-positive (P < .001), compared with 64.3% (n = 36/56) of MCPP cases and 6.3% (n = 243/3832) of nonconfirmed cases (P < .001). Blood pneumococcal PCR positivity was higher in children from the 5 African countries (5.5%-11.5% among cases and 5.3%-10.2% among controls) than from the 2 Asian countries (1.3% and 1.0% among cases and 0.8% and 0.8% among controls). Among Kilifi general pediatric admissions, 3.9% (n = 274/6968) were PCR-positive, including 61.7% (n = 37/60) of those with positive blood cultures for pneumococcus. Discussion. The utility of pneumococcal PCR on blood for diagnosing childhood pneumococcal pneumonia in the 7 low- and middle-income countries studied is limited by poor specificity and by poor sensitivity among MCPP cases.

Original language	English
Pages (from-to)	S347-S356
Journal	Clinical Infectious Diseases
Volume	64
DOIs	https://doi.org/10.1093/cid/cix145
Publication status	Published - 1 Jan 2017
Externally published	Yes

Keywords

Blood
Diagnosis
PCR
Pneumococcus
Pneumonia

Access to Document

10.1093/cid/cix145

Cite this

Morpeth, S. C., Knoll, M. D., Scott, J. A. G., Park, D. E., Watson, N. L., Baggett, H. C., Brooks, W. A., Feikin, D. R., Hammitt, L. L., Howie, S. R. C., Kotloff, K. L., Levine, O. S., Madhi, S. A., O'Brien, K. L., Thea, D. M., Adrian, P. V., Ahmed, D., Antonio, M., Bunthi, C., ... Kamau, A. (2017). Detection of pneumococcal DNA in blood by polymerase chain reaction for diagnosing pneumococcal pneumonia in young children from low- and middle-income countries. Clinical Infectious Diseases, 64, S347-S356. https://doi.org/10.1093/cid/cix145

@article{580c801cff9c47c7856024d3ef05415f,

title = "Detection of pneumococcal DNA in blood by polymerase chain reaction for diagnosing pneumococcal pneumonia in young children from low- and middle-income countries",

abstract = "Background. We investigated the performance of polymerase chain reaction (PCR) on blood in the diagnosis of pneumococcal pneumonia among children from 7 low- and middle-income countries. Methods. We tested blood by PCR for the pneumococcal autolysin gene in children aged 1-59 months in the Pneumonia Etiology Research for Child Health (PERCH) study. Children had World Health Organization-defined severe or very severe pneumonia or were age-frequency-matched community controls. Additionally, we tested blood from general pediatric admissions in Kilifi, Kenya, a PERCH site. The proportion PCR-positive was compared among cases with microbiologically confirmed pneumococcal pneumonia (MCPP), cases without a confirmed bacterial infection (nonconfirmed), cases confirmed for nonpneumococcal bacteria, and controls. Results. In PERCH, 7.3\% (n = 291/3995) of cases and 5.5\% (n = 273/4987) of controls were blood pneumococcal PCR-positive (P < .001), compared with 64.3\% (n = 36/56) of MCPP cases and 6.3\% (n = 243/3832) of nonconfirmed cases (P < .001). Blood pneumococcal PCR positivity was higher in children from the 5 African countries (5.5\%-11.5\% among cases and 5.3\%-10.2\% among controls) than from the 2 Asian countries (1.3\% and 1.0\% among cases and 0.8\% and 0.8\% among controls). Among Kilifi general pediatric admissions, 3.9\% (n = 274/6968) were PCR-positive, including 61.7\% (n = 37/60) of those with positive blood cultures for pneumococcus. Discussion. The utility of pneumococcal PCR on blood for diagnosing childhood pneumococcal pneumonia in the 7 low- and middle-income countries studied is limited by poor specificity and by poor sensitivity among MCPP cases.",

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

author = "Morpeth, \{Susan C.\} and Knoll, \{Maria Deloria\} and Scott, \{J. Anthony G.\} and Park, \{Daniel E.\} and Watson, \{Nora L.\} 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 Madhi, \{Shabir A.\} and O'Brien, \{Katherine L.\} and Thea, \{Donald M.\} and Adrian, \{Peter V.\} and Dilruba Ahmed and Martin Antonio and Charatdao Bunthi and DeLuca, \{Andrea N.\} and Driscoll, \{Amanda J.\} and Githua, \{Louis Peter\} and Higdon, \{Melissa M.\} and Geoff Kahn and Angela Karani and Karron, \{Ruth A.\} and Geoffrey Kwenda and Sirirat Makprasert and Razib Mazumder and Moore, \{David P.\} and James Mwansa and Sammy Nyongesa and Christine Prosperi and Sow, \{Samba O.\} and Boubou Tamboura and Toni Whistler and Zeger, \{Scott L.\} and Murdoch, \{David R.\} 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 Alice Kamau",

year = "2017",

month = jan,

day = "1",

doi = "10.1093/cid/cix145",

language = "English",

volume = "64",

pages = "S347--S356",

journal = "Clinical Infectious Diseases",

issn = "1058-4838",

publisher = "Oxford University Press",

}

Morpeth, SC, Knoll, MD, Scott, JAG, Park, DE, Watson, NL, Baggett, HC, Brooks, WA, Feikin, DR, Hammitt, LL, Howie, SRC, Kotloff, KL, Levine, OS, Madhi, SA, O'Brien, KL, Thea, DM, Adrian, PV, Ahmed, D, Antonio, M, Bunthi, C, DeLuca, AN, Driscoll, AJ, Githua, LP, Higdon, MM, Kahn, G, Karani, A, Karron, RA, Kwenda, G, Makprasert, S, Mazumder, R, Moore, DP, Mwansa, J, Nyongesa, S, Prosperi, C, Sow, SO, Tamboura, B, Whistler, T, Zeger, SL, Murdoch, DR, Fancourt, N, Fu, W, Kagucia, EW, Li, M, Wu, Z, Crawley, J, Endtz, HP, Zaman, K, Goswami, D, Hossain, L, Jahan, Y & Kamau, A 2017, 'Detection of pneumococcal DNA in blood by polymerase chain reaction for diagnosing pneumococcal pneumonia in young children from low- and middle-income countries', Clinical Infectious Diseases, vol. 64, pp. S347-S356. https://doi.org/10.1093/cid/cix145

Detection of pneumococcal DNA in blood by polymerase chain reaction for diagnosing pneumococcal pneumonia in young children from low- and middle-income countries. / Morpeth, Susan C.; Knoll, Maria Deloria; Scott, J. Anthony G. et al.
In: Clinical Infectious Diseases, Vol. 64, 01.01.2017, p. S347-S356.

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

TY - JOUR

T1 - Detection of pneumococcal DNA in blood by polymerase chain reaction for diagnosing pneumococcal pneumonia in young children from low- and middle-income countries

AU - Morpeth, Susan C.

AU - Knoll, Maria Deloria

AU - Scott, J. Anthony G.

AU - Park, Daniel E.

AU - Watson, Nora L.

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 - Madhi, Shabir A.

AU - O'Brien, Katherine L.

AU - Thea, Donald M.

AU - Adrian, Peter V.

AU - Ahmed, Dilruba

AU - Antonio, Martin

AU - Bunthi, Charatdao

AU - DeLuca, Andrea N.

AU - Driscoll, Amanda J.

AU - Githua, Louis Peter

AU - Higdon, Melissa M.

AU - Kahn, Geoff

AU - Karani, Angela

AU - Karron, Ruth A.

AU - Kwenda, Geoffrey

AU - Makprasert, Sirirat

AU - Mazumder, Razib

AU - Moore, David P.

AU - Mwansa, James

AU - Nyongesa, Sammy

AU - Prosperi, Christine

AU - Sow, Samba O.

AU - Tamboura, Boubou

AU - Whistler, Toni

AU - Zeger, Scott L.

AU - Murdoch, David R.

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 - Kamau, Alice

PY - 2017/1/1

Y1 - 2017/1/1

N2 - Background. We investigated the performance of polymerase chain reaction (PCR) on blood in the diagnosis of pneumococcal pneumonia among children from 7 low- and middle-income countries. Methods. We tested blood by PCR for the pneumococcal autolysin gene in children aged 1-59 months in the Pneumonia Etiology Research for Child Health (PERCH) study. Children had World Health Organization-defined severe or very severe pneumonia or were age-frequency-matched community controls. Additionally, we tested blood from general pediatric admissions in Kilifi, Kenya, a PERCH site. The proportion PCR-positive was compared among cases with microbiologically confirmed pneumococcal pneumonia (MCPP), cases without a confirmed bacterial infection (nonconfirmed), cases confirmed for nonpneumococcal bacteria, and controls. Results. In PERCH, 7.3% (n = 291/3995) of cases and 5.5% (n = 273/4987) of controls were blood pneumococcal PCR-positive (P < .001), compared with 64.3% (n = 36/56) of MCPP cases and 6.3% (n = 243/3832) of nonconfirmed cases (P < .001). Blood pneumococcal PCR positivity was higher in children from the 5 African countries (5.5%-11.5% among cases and 5.3%-10.2% among controls) than from the 2 Asian countries (1.3% and 1.0% among cases and 0.8% and 0.8% among controls). Among Kilifi general pediatric admissions, 3.9% (n = 274/6968) were PCR-positive, including 61.7% (n = 37/60) of those with positive blood cultures for pneumococcus. Discussion. The utility of pneumococcal PCR on blood for diagnosing childhood pneumococcal pneumonia in the 7 low- and middle-income countries studied is limited by poor specificity and by poor sensitivity among MCPP cases.

AB - Background. We investigated the performance of polymerase chain reaction (PCR) on blood in the diagnosis of pneumococcal pneumonia among children from 7 low- and middle-income countries. Methods. We tested blood by PCR for the pneumococcal autolysin gene in children aged 1-59 months in the Pneumonia Etiology Research for Child Health (PERCH) study. Children had World Health Organization-defined severe or very severe pneumonia or were age-frequency-matched community controls. Additionally, we tested blood from general pediatric admissions in Kilifi, Kenya, a PERCH site. The proportion PCR-positive was compared among cases with microbiologically confirmed pneumococcal pneumonia (MCPP), cases without a confirmed bacterial infection (nonconfirmed), cases confirmed for nonpneumococcal bacteria, and controls. Results. In PERCH, 7.3% (n = 291/3995) of cases and 5.5% (n = 273/4987) of controls were blood pneumococcal PCR-positive (P < .001), compared with 64.3% (n = 36/56) of MCPP cases and 6.3% (n = 243/3832) of nonconfirmed cases (P < .001). Blood pneumococcal PCR positivity was higher in children from the 5 African countries (5.5%-11.5% among cases and 5.3%-10.2% among controls) than from the 2 Asian countries (1.3% and 1.0% among cases and 0.8% and 0.8% among controls). Among Kilifi general pediatric admissions, 3.9% (n = 274/6968) were PCR-positive, including 61.7% (n = 37/60) of those with positive blood cultures for pneumococcus. Discussion. The utility of pneumococcal PCR on blood for diagnosing childhood pneumococcal pneumonia in the 7 low- and middle-income countries studied is limited by poor specificity and by poor sensitivity among MCPP cases.

KW - Blood

KW - Diagnosis

KW - PCR

KW - Pneumococcus

KW - Pneumonia

U2 - 10.1093/cid/cix145

DO - 10.1093/cid/cix145

M3 - Article

SN - 1058-4838

VL - 64

SP - S347-S356

JO - Clinical Infectious Diseases

JF - Clinical Infectious Diseases

ER -

Detection of pneumococcal DNA in blood by polymerase chain reaction for diagnosing pneumococcal pneumonia in young children from low- and middle-income countries

Abstract

Keywords

Access to Document

Fingerprint

Cite this