DETEKSI GEN ENTEROTOKSIN G dan I Staphylococcus aureus DARI SUSU NORMAL, MASTITIS SUBKLINIS DAN MASTITIS KLINIS DENGAN TEKNIK Multiplex Polymerase Chain Reaction
Mastitis is an abnormality in mammary gland causing a great loss of milk production. One of the frequent bacteria that inflict this disease is Staphylococcus aureus, which can also produce toxin then lead to food toxicity and gastroenteritis. This toxin is one of important virulence...
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| Main Authors: | , |
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| Format: | Theses and Dissertations NonPeerReviewed |
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[Yogyakarta] : Universitas Gadjah Mada
2014
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| Online Access: | https://repository.ugm.ac.id/130639/ http://etd.ugm.ac.id/index.php?mod=penelitian_detail&sub=PenelitianDetail&act=view&typ=html&buku_id=71065 |
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| Institution: | Universitas Gadjah Mada |
| Summary: | Mastitis is an abnormality in mammary gland causing a great loss of milk
production. One of the frequent bacteria that inflict this disease is Staphylococcus
aureus, which can also produce toxin then lead to food toxicity and
gastroenteritis. This toxin is one of important virulence factor in Staphylococcus
aureus called Staphylococcal Enterotoxin (SE). In order to detect the presence of
enterotoxin coding gene which can be in various type, the use of Multiplex
Polymerase Chain Reaction which can detect more than one sequence target using
two pair of primers or more in a reaction can detect the presence of enterotoxin
coding gene faster than any other method.
Various type of enterotoxin had been identified, SEA-A, and SEG-V, also
SEG and SEI which had high morbidity rate in bovine mastitis case. Thirty two
(32) isolates of Staphylococcus aureus from milk taken from dairy farm in
Boyolali, Pacitan, and Ponorogo, were detected in presence of segandseigene.
Reidentification of S. aureus by culturing the bacteria in Blood Agarose Plate
(BAP), Gram stain, Catalase test, Coagulation Test, Mannitol Salt Agar (MSA),
and VogesProuskauer (VP) Test. Molecular detection of 23S rRNA gene to
identify S. aureus by Polymerase Chain Reaction (PCR) was done using specific
primer 5�-ACGGAGTTACAAAGGACGAC-3� (forward) and 5�-AGCTCAGCCTTAACGAGTAC-3� (reverse) resulting in 1250 bp of
amplification product. The primer for the detection of segand sei coding gene was
designed for multiplex PCR method using MP Primer software. The primer for
seg gene 5'-TGAATTATGTGAATGCTCAACCCG-3' (forward) and 5'-GCAGAACCATCAAACTCGTATAGC-3' (reverse) with amplification product
of 541 bp.For the sei gene 5'-ACCTACCTATTGCAAATCAACTCG-3' (forward)
and 5'-CCATATTCTTTGCCTTTACCAGTGT-3' (reverse) resulting in 373 bp of
amplification product.
The result showed thirty two (32) isolates were Staphylococcus aureus in
23s rRNA gene and from the sequence result. The results in the detection of seg
and sei coding gene showed 28 (87.5%) positive sample in Boyolali, Pacitan, and
Ponorogo. From 87.5% positive sample, 9.37% were seg positive, 34.37% were
sei positive, and 43.75% were seg and sei positive. According to the result
sequence, the seg gene had 99% similarity with S.aureus Accession number
AY920262.1, and the sei gene had 99% similarity with S.aureus Accession
number AY961382.1. Subclinical mastitis milk containing 3.7% seg gene, 37.08%
sei, 44.44% se (g, i) and 14.8% negative, clinical mastitis milk containing 100%
sei, and normal milk containing 50% seg and 50% se(g, i). |
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