Details der Publikation - Rapid detection of Pseudomonas aeruginosa targeting the toxA gene in intensive care unit patients from Beijing, China

Rapid detection of Pseudomonas aeruginosa targeting the toxA gene in intensive care unit patients from Beijing, China

Pseudomonas aeruginosa is a major opportunistic pathogen in hospital-acquired infections and exhibits increasing antibiotic resistance. A rapid and sensitive molecular method for its detection in clinical samples is needed to guide therapeutic treatment and to control P. aeruginosa outbreaks. In this study, we established a polymerase spiral reaction (PSR) method for rapid detection of P. aeruginosa by targeting the toxA gene, which regulates exotoxin A synthesis. Real-time turbidity monitoring and a chromogenic visualization using hydroxynaphthol blue were used to assess the reaction. All 17 non- P. aeruginosa strains tested negative, indicating the high specificity of the PSR primers. The detection limit was 2.3 pg/µl within 60 min at isothermal temperature (65°C), 10-fold more sensitive than conventional PCR. Then, the PSR assay was applied to a clinical surveillance of P. aeruginosa in three top hospitals in Beijing, China. Of the 130 sputum samples collected from ICU patients with suspected multi-resistant infections, 37 P. aeruginosa isolates were identified from the positive samples. All clinical strains belonged to 10 different P. aeruginosa multilocus sequence typing groups and exhibited high resistance to carbapenems, cephalosporins, and aminoglycosides. Interestingly, of the 33 imipenem-resistant isolates, 30 (90.9%) had lost the outer membrane porin oprD gene. Moreover, isolate SY-95, containing multiple antibiotic resistance genes, possessed the ability to hydrolyze all antibiotics used in clinic and was susceptible only to polymyxin B. Our study showed the high level of antibiotic resistance and co-occurrence of resistance genes in the clinical strains, indicating a rapid and continuing evolution of P. aeruginosa. In conclusion, we developed a P. aeruginosa PSR assay, which could be a useful tool for clinical screening, especially in case of poor resources, or for point-of-care testing..

Medienart:	E-Artikel

Erscheinungsjahr:	2015
Erschienen:	2015

Enthalten in:	Zur Gesamtaufnahme - volume:6
Enthalten in:	Frontiers in Microbiology - 6(2015)

Sprache:	Englisch

Beteiligte Personen:	Derong eDong [VerfasserIn] Dayang eZou [VerfasserIn] Hui eLiu [VerfasserIn] Zhan eYang [VerfasserIn] Simo eHuang [VerfasserIn] Ningwei eLiu [VerfasserIn] Xiaoming eHe [VerfasserIn] Wei eLiu [VerfasserIn] Liuyu eHuang [VerfasserIn]

Links:	doi.org [kostenfrei] doaj.org [kostenfrei] journal.frontiersin.org [kostenfrei] Journal toc [kostenfrei]

Themen:	ETA Isothermal Microbiology P. aeruginosa PSR Rapid diagnosis

doi:	10.3389/fmicb.2015.01100

funding:
Förderinstitution / Projekttitel:

PPN (Katalog-ID):	DOAJ060024569

Internformat


LEADER	01000caa a22002652 4500
001	DOAJ060024569
003	DE-627
005	20230309000536.0
007	cr uuu---uuuuu
008	230228s2015 xx \|\|\|\|\|o 00\| \|\|eng c
024	7		\|a 10.3389/fmicb.2015.01100 \|2 doi
035			\|a (DE-627)DOAJ060024569
035			\|a (DE-599)DOAJ94f5bdf91095459c9bae8e0566dacfb9
040			\|a DE-627 \|b ger \|c DE-627 \|e rakwb
041			\|a eng
050		0	\|a QR1-502
100	0		\|a Derong eDong \|e verfasserin \|4 aut
245	1	0	\|a Rapid detection of Pseudomonas aeruginosa targeting the toxA gene in intensive care unit patients from Beijing, China
264		1	\|c 2015
336			\|a Text \|b txt \|2 rdacontent
337			\|a Computermedien \|b c \|2 rdamedia
338			\|a Online-Ressource \|b cr \|2 rdacarrier
520			\|a Pseudomonas aeruginosa is a major opportunistic pathogen in hospital-acquired infections and exhibits increasing antibiotic resistance. A rapid and sensitive molecular method for its detection in clinical samples is needed to guide therapeutic treatment and to control P. aeruginosa outbreaks. In this study, we established a polymerase spiral reaction (PSR) method for rapid detection of P. aeruginosa by targeting the toxA gene, which regulates exotoxin A synthesis. Real-time turbidity monitoring and a chromogenic visualization using hydroxynaphthol blue were used to assess the reaction. All 17 non- P. aeruginosa strains tested negative, indicating the high specificity of the PSR primers. The detection limit was 2.3 pg/µl within 60 min at isothermal temperature (65°C), 10-fold more sensitive than conventional PCR. Then, the PSR assay was applied to a clinical surveillance of P. aeruginosa in three top hospitals in Beijing, China. Of the 130 sputum samples collected from ICU patients with suspected multi-resistant infections, 37 P. aeruginosa isolates were identified from the positive samples. All clinical strains belonged to 10 different P. aeruginosa multilocus sequence typing groups and exhibited high resistance to carbapenems, cephalosporins, and aminoglycosides. Interestingly, of the 33 imipenem-resistant isolates, 30 (90.9%) had lost the outer membrane porin oprD gene. Moreover, isolate SY-95, containing multiple antibiotic resistance genes, possessed the ability to hydrolyze all antibiotics used in clinic and was susceptible only to polymyxin B. Our study showed the high level of antibiotic resistance and co-occurrence of resistance genes in the clinical strains, indicating a rapid and continuing evolution of P. aeruginosa. In conclusion, we developed a P. aeruginosa PSR assay, which could be a useful tool for clinical screening, especially in case of poor resources, or for point-of-care testing.
650		4	\|a P. aeruginosa
650		4	\|a rapid diagnosis
650		4	\|a Isothermal
650		4	\|a PSR
650		4	\|a ETA
653		0	\|a Microbiology
700	0		\|a Dayang eZou \|e verfasserin \|4 aut
700	0		\|a Hui eLiu \|e verfasserin \|4 aut
700	0		\|a Zhan eYang \|e verfasserin \|4 aut
700	0		\|a Simo eHuang \|e verfasserin \|4 aut
700	0		\|a Ningwei eLiu \|e verfasserin \|4 aut
700	0		\|a Xiaoming eHe \|e verfasserin \|4 aut
700	0		\|a Wei eLiu \|e verfasserin \|4 aut
700	0		\|a Liuyu eHuang \|e verfasserin \|4 aut
773	0	8	\|i In \|t Frontiers in Microbiology \|d Frontiers Media S.A., 2011 \|g 6(2015) \|w (DE-627)DOAJ000031836 \|x 1664302X \|7 nnns
773	1	8	\|g volume:6 \|g year:2015
856	4	0	\|u https://doi.org/10.3389/fmicb.2015.01100 \|z kostenfrei
856	4	0	\|u https://doaj.org/article/94f5bdf91095459c9bae8e0566dacfb9 \|z kostenfrei
856	4	0	\|u http://journal.frontiersin.org/Journal/10.3389/fmicb.2015.01100/full \|z kostenfrei
856	4	2	\|u https://doaj.org/toc/1664-302X \|y Journal toc \|z kostenfrei
912			\|a GBV_USEFLAG_A
912			\|a GBV_DOAJ
951			\|a AR
952			\|d 6 \|j 2015

Rapid detection of Pseudomonas aeruginosa targeting the toxA gene in intensive care unit patients from Beijing, China

Zugang & Verfügbarkeit

Zugehörige Publikationen/Bände