QCM-based rapid detection of PCR amplification products of Ehrlichia canis

Bunroddith K.; Viseshakul N.; Chansiri K.; Lieberzeit P.

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dc.contributor.author	Bunroddith K.
dc.contributor.author	Viseshakul N.
dc.contributor.author	Chansiri K.
dc.contributor.author	Lieberzeit P.
dc.date.accessioned	2021-04-05T03:21:37Z
dc.date.available	2021-04-05T03:21:37Z
dc.date.issued	2018
dc.identifier.issn	32670
dc.identifier.other	2-s2.0-85035109804
dc.identifier.uri	https://ir.swu.ac.th/jspui/handle/123456789/12798
dc.identifier.uri	https://www.scopus.com/inward/record.uri?eid=2-s2.0-85035109804&doi=10.1016%2fj.aca.2017.10.037&partnerID=40&md5=c8dcfbab9472bcdeec900d30d861324b
dc.description.abstract	Ehrlichia canis is an intracellular parasitic bacterium and arthropod-borne pathogen that receives growing attention, because it leads to increasing morbidity and mortality in animals. It does so by causing canine monocytotropic ehrlichiosis (CME). Infected canines may lack obvious clinical signs and stay in chronic stage. Herein we report a rapid screening method based on PCR assay combined with quartz crystal microbalance (QCM) to design a DNA sensor for detecting E. canis in early stages of infection. The test relies on DNA amplification of target nucleotide sequences via PCR followed by detecting DNA-DNA hybridization using QCM. The approach did not result in any cross-hybridization toward other blood bacteria or parasites in dogs, such as Anaplasma platys, Babesia canis and Trypanosoma spp, but turned out selective for the target species. The limit of detection of QCM was as low as 4.1 × 109 molecules/μl of 289 bp E. canis PCR products corresponding to 22 copy numbers/μl of E. canis. Furthermore, the technique is also simple, does not require complicated equipment and can in principle be reused. © 2017 Elsevier B.V.
dc.subject	Bacteria
dc.subject	DNA
dc.subject	DNA sequences
dc.subject	Quartz
dc.subject	Quartz crystal microbalances
dc.subject	Cross hybridization
dc.subject	DNA amplification
dc.subject	DNA biosensors
dc.subject	DNA-DNA hybridization
dc.subject	Ehrlichia canis
dc.subject	Limit of detection
dc.subject	Nucleotide sequences
dc.subject	PCR amplification
dc.subject	Polymerase chain reaction
dc.subject	Article
dc.subject	bacterium detection
dc.subject	blood sampling
dc.subject	controlled study
dc.subject	copy number variation
dc.subject	cross hybridization
dc.subject	DNA hybridization
dc.subject	Ehrlichia canis
dc.subject	gene amplification
dc.subject	immobilization
dc.subject	limit of detection
dc.subject	molecular probe
dc.subject	nonhuman
dc.subject	nucleotide sequence
dc.subject	polymerase chain reaction
dc.subject	priority journal
dc.subject	process optimization
dc.subject	quartz crystal microbalance
dc.subject	screening test
dc.subject	animal
dc.subject	devices
dc.subject	dog
dc.subject	dog disease
dc.subject	Ehrlichia canis
dc.subject	ehrlichiosis
dc.subject	equipment design
dc.subject	genetics
dc.subject	isolation and purification
dc.subject	microbiology
dc.subject	polymerase chain reaction
dc.subject	procedures
dc.subject	quartz crystal microbalance
dc.subject	veterinary
dc.subject	bacterial DNA
dc.subject	Animals
dc.subject	DNA, Bacterial
dc.subject	Dog Diseases
dc.subject	Dogs
dc.subject	Ehrlichia canis
dc.subject	Ehrlichiosis
dc.subject	Equipment Design
dc.subject	Limit of Detection
dc.subject	Polymerase Chain Reaction
dc.subject	Quartz Crystal Microbalance Techniques
dc.title	QCM-based rapid detection of PCR amplification products of Ehrlichia canis
dc.type	Article
dc.rights.holder	Scopus
dc.identifier.bibliograpycitation	Analytica Chimica Acta. Vol 1001, (2018), p.106-111
dc.identifier.doi	10.1016/j.aca.2017.10.037