Literature DB >> 9709219

Detection of bovine mitochondrial DNA in ruminant feeds: a molecular approach to test for the presence of bovine-derived materials.

M Tartaglia1, E Saulle, S Pestalozza, L Morelli, G Antonucci, P A Battaglia.   

Abstract

A ban on ruminant-derived proteins in ruminant feeds has been introduced as a preventive measure to avoid the spread of bovine spongiform encephalopathy (BSE), as well as to minimize any potential risk of BSE transmission from bovines to humans. In the absence of commercially available efficient methods for identification of bovine-derived proteins in animal feeds, we developed a rapid and sensitive polymerase chain reaction (PCR)-based assay which allows detection and identification of a bovine-specific mitochondrial DNA sequence from feedstuffs. The amplified product encodes for the whole ATPase subunit 8 and the amino-terminal portion of the ATPase subunit 6 proteins, which are known to exhibit a relatively low degree of conservation among vertebrates. The specific amplification of such a bovine mitochondrial sequence from reference feedstuff samples was demonstrated by means of both direct sequencing and single-strand conformational analysis of the PCR product. Specificity was also confirmed by the absence of detectable homologous PCR product when using reference feedstuff samples lacking bovine-derived meat and bonemeals, or genomic DNA samples from vertebrates whose offals are commonly included in animal feeds. This method allows detection of the presence of bovine mitochondrial DNA in feedstuffs containing less than 0.125% of bovine-derived meat and bonemeals. Furthermore, it does not appear to be considerably affected by prolonged heat treatment. DpnII and SspI restriction endonuclease digestions of the unpurified PCR product may be used routinely to confirm the bovine origin of the amplified sequence. Since this method is specific, rapid, and sensitive, it could be successfully utilized as a routine control assay to evaluate the presence of bovine-derived meat and bonemeals in ruminant feeds.

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Year:  1998        PMID: 9709219     DOI: 10.4315/0362-028x-61.5.513

Source DB:  PubMed          Journal:  J Food Prot        ISSN: 0362-028X            Impact factor:   2.077


  10 in total

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Journal:  Vet Res Commun       Date:  2003-09       Impact factor: 2.459

2.  Detection of genetically modified organisms (GMOs) in food and feedstuff.

Authors:  E Novelli; S Balzan; S Segato; L De Rigo; M Ferioli
Journal:  Vet Res Commun       Date:  2003-09       Impact factor: 2.459

3.  A preliminary trial using multi-target polymerase chain reaction (multiplex PCR) and restriction fragment length polymorphism (PCR-RFLP) on the same feedstuffs to detect tissues of animal origin.

Authors:  F Colombo; E Marchisio; I E Trezzi; V Peri; L Pinotti; A Baldi; G Soncini
Journal:  Vet Res Commun       Date:  2004-08       Impact factor: 2.459

4.  Development of species identification tests targeting the 16S ribosomal RNA coding region in mitochondrial DNA.

Authors:  Kazuhiko Imaizumi; Tomoko Akutsu; Sachio Miyasaka; Mineo Yoshino
Journal:  Int J Legal Med       Date:  2006-11-16       Impact factor: 2.686

5.  Identification of pork in meat products using real-time loop-mediated isothermal amplification.

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Authors:  M Mansoor Bhat; Mir Salahuddin; Imtiyaz A Mantoo; Sheikh Adil; Henna Jalal; M Ashraf Pal
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7.  Droplet digital polymerase chain reaction (ddPCR) assays integrated with an internal control for quantification of bovine, porcine, chicken and turkey species in food and feed.

Authors:  Hanan R Shehata; Jiping Li; Shu Chen; Helen Redda; Shumei Cheng; Nicole Tabujara; Honghong Li; Keith Warriner; Robert Hanner
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Authors:  Nining Irfanita; Widya Lestari; Mohamed Elwathig Saeed Mirghani; Irwandi Jaswir; Fitri Octavianti; Muhammad Salahuddin Haris
Journal:  Trop Life Sci Res       Date:  2022-07-15

10.  Development of loop-mediated isothermal amplification (LAMP) assay for rapid and sensitive identification of ostrich meat.

Authors:  Amir Abdulmawjood; Nils Grabowski; Svenja Fohler; Sophie Kittler; Helga Nagengast; Guenter Klein
Journal:  PLoS One       Date:  2014-06-25       Impact factor: 3.240

  10 in total

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