molecular typing of brucella melitensis and b. abortus from human blood samples using pcr-rflp method

Authors

reza mirnejad molecular biology research center, baqiyatallah university of medical sciences, tehran, ir iran

mozafar mohammadi molecular biology research center, baqiyatallah university of medical sciences, tehran, ir iran

ali majdi young researchers club, tonekabon branch, islamic azad university, tonekabon, ir iran

niloufar taghizoghi bounty house, stowage, bellerbys college, london, united kingdom

abstract

conclusions the results of this study showed that pcr–rflp technique was a fast and applicable method especially for separation, detection and differentiation between species of b. melitensis and b. abortus biovars in blood sample. also the presented data showed that b. melitensis biovar 1 was the prevalence biovar. background brucella is an intracellular parasite of the disease brucellosis throughout the world. although several molecular typing methods are introduced to find dna polymorphism that is able to identify brucella species and biovars, but among these methods, detection of polymorphisms by pcr–rflp has several advantages including the easy implementation, interpretation and the ease of use for large quantities of samples. objectives in the current study, the technique was used for molecular typing of brucella abortus and b. melitensis that was isolated from human blood samples. materials and methods blood samples of 160 patients were transferred to kerman clinical centers with chief complain of acute brucellosis and showed high blood serum level (about 1.80). their dnas were extracted by phenol chloroform method, and the pcr was optimized by using the fragments of designed primers for omp2a and omp2b. therefore pcr products were restricted by restriction endonuclease as psti and hinf1. finally they were electrophoresed for analyzing the digestion results on agarose gels (2%). results in 160 blood samples that were studied with pcr technique, 52 cases obtained bands of 1100 bp for omp2a locus and 1200 bp for omp2b locus from within 52 positive samples by pcr–rflp method 25 cases (48%) were positive out of which 56% were b. melitensis biovar1 and 44% were b. abortus biovars of 3, 5, 6 or 9.

Upgrade to premium to download articles

Sign up to access the full text

Already have an account?login

similar resources

Detection of Brucella melitensis and Brucella abortus strains using a single-stage PCR method

  Brucella melitensis and Brucella abortus are of the most important causes of brucellosis, an infectious disease which is transmitted either directly or indirectly including consuming unpasteurized dairy products. Both strains are considered endemic in Iran. Common diagnostic methods such as bacteriologic cultures are difficult and time consuming regarding the bacteria. The aim of this study w...

full text

MLVA16 Typing of Portuguese Human and Animal Brucella melitensis and Brucella abortus Isolates

To investigate the epidemiological relationship of isolates from different Portuguese geographical regions and to assess the diversity among isolates, the MLVA16(Orsay) assay (panels 1, 2A and 2B) was performed with a collection of 126 Brucella melitensis (46 human and 80 animal isolates) and 157 B. abortus field isolates, seven vaccine strains and the representative reference strains of each s...

full text

detection of brucella melitensis and brucella abortus strains using a single-stage pcr method

brucella melitensis and brucella abortus are of the most important causes of brucellosis, an infectious disease which is transmitted either directly or indirectly including consuming unpasteurized dairy products. both strains are considered endemic in iran. common diagnostic methods such as bacteriologic cultures are difficult and time consuming regarding the bacteria. the aim of this study was...

full text

Real-time multiplex PCR assay for detection of Brucella spp., B. abortus, and B. melitensis.

The identification of Brucella can be a time-consuming and labor-intensive process that places personnel at risk for laboratory-acquired infection. Here, we describe a real-time PCR assay for confirmation of presumptive Brucella isolates. The assay was designed in a multiplex format that will allow the rapid identification of Brucella spp., B. abortus, and B. melitensis in a single test.

full text

A Novel PCR Assay for Detecting Brucella abortus and Brucella melitensis

OBJECTIVES Brucellosis is a major zoonotic disease that poses a significant public health threat worldwide. The classical bacteriological detection process used to identify Brucella spp. is difficult and time-consuming. This study aimed to develop a novel molecular assay for detecting brucellosis. METHODS All complete sequences of chromosome 1 with 2.1-Mbp lengths were compared among all avai...

full text

Rapid multiplex PCR assay for the simultaneous detection of the Brucella Genus, B. abortus, B. melitensis, and B. suis.

The routine identification and differentiation of Brucella species is a time-consuming and labor-intensive process, which frequently places personnel at risk of laboratoryacquired infection. Here, we describe the development of a rapid multiplex PCR assay for the confirmation of presumptive Brucella isolates. The assay was able to identify and differentiate major human pathogens, namely B. abor...

full text

My Resources

Save resource for easier access later


Journal title:
jundishapur journal of microbiology

جلد ۶، شماره ۶، صفحات ۰-۰

Hosted on Doprax cloud platform doprax.com

copyright © 2015-2023