Citation
Lim, Sor Sing
(2005)
Application of Polymerase Chain Reaction Restriction Fragment Length Polymorphism Technique in Determining the Identity of Several Marine Species in Seafood Products.
Masters thesis, Universiti Putra Malaysia.
Abstract
This study describes an investigation on the application of Polymerase Chain
Reaction-Restriction Fragment Length Polymorphism (PCR-RFLP) nucleic acid
based technique, as a routine analytical technique to generate DNA fingerprints for
24 fresh marine samples. Data obtained from the DNA fingerprints were used to
identify 12 processed marine samples. Samples representative of various species and
marine products submitted to different processing conditions were selected to verify
the applicability of the techniques. A specific part of mitochondrion (mt) genome,
cytochrome b (cytb) gene with 359 base pair (bp) fragment was successfully
amplified from all the investigated samples by using ‘universal’ primer pairs. The
obtained fragment of cytb gene (359 bp) was digested with different Restriction
Endonuclease (RE) resulting in sample specific Restriction Fragment Length
Polymorphism (RFLP). A total of 14 fishes, 7 prawns and 3 crabs with the exception
of Doublelined tonguesole (Paraplagusia bilineata), Rainbow sardine (Dussumieria
acuta), Western king prawn (Metapenaeus latisulcatus), Sharp-rostrum prawn
(Parapenaeopsis hardwickii), Giant freshwater prawn (Macrobrachium
rosenbergii), Affluent prawn (Thenus orientalis), Giant tiger prawn (Penaeus semisulcatus), Indo-pacific swamp crab (Scylla serrata), Red and Blue swimming
crab (Solenocera subnuda) could be differentiated using RE HaeIII, MboII, FokI,
and MspI followed by agarose gel electrophoresis. For processed marine samples,
only four out of twelve were successfully identified. The DNA of unidentifiable
samples may have been degraded during the steps of processing. The RFLP patterns
obtained are conclusive even in the mixture of Western king prawn (Metapenaeus
latisulcatus) and African threadfin (Alexis alexandrinus) at a ratio of 1:100. Results
of this study suggest that the PCR-RFLP based on cytb gene shows a reproducible,
rapid and simple method for simultaneous identification of marine samples.
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