Development of a Multiplex Polymerase Chain Reaction Method for Rapid and Accurate Identification of Girella punctata and G. leonina (Teleostei: Girellidae)

Author:

Kim Eun-Mi1ORCID,Lee Mi-Nan1,Dong Chun-Mae1,Noh Jae-Koo2,Noh Eun-Soo1,Kim Woo-Jin1,Nam Bo-Hye3,Kim Young-Ok1

Affiliation:

1. Biotechnology Research Division, National Institute of Fisheries Science, Busan 46083, Republic of Korea

2. Subtropical Fisheries Research Institute, National Institute of Fisheries Science, Jeju 63068, Republic of Korea

3. Aquaculture Management Division, National Institute of Fisheries Science, Busan 46083, Republic of Korea

Abstract

Girella punctata and Girella leonina are economically important species found in the East Sea; along the southern coast of Korea; south of Hokkaido, Japan; around Taiwan; and in the East China sea. In Korea, these two species hold high value, particularly on Jeju Island. These species have similar appearances, and it is challenging to distinguish them, particularly during the seed period. We detected genetic differences in the mtDNA (COI gene) of G. punctata and G. leonina, which are morphologically indistinguishable, and developed species-specific genetic markers for their identification. In total, 16 and 4 haplotypes of the COI genes were obtained from G. punctata (n = 164) and G. leonina (n = 36), respectively. The haplotype diversity (Hd) and nucleotide diversity (Pi, %) of the COI were 0.359 and 0.054 for G. punctata and 0.560 and 0.078 for G. leonina, respectively. We designed a Girella species common primer (control) and species-specific primer sets (experimental) for the two species. Amplicon sizes of 991, 579, and 391 bp were obtained for common primers of the two Girella species G. punctata and G. leonina. To confirm multiple targets in a single reaction, multiplex PCR conditions were optimized to adjust its resolution and accuracy. The detection levels of the multiplex PCR were confirmed to be 0.01 ng/µL for the two Girella species. The multiplex PCR was not associated with cross-reactivity between G. punctata and G. leonina. This multiplex species-specific PCR method provides a simple and rapid technique for the identification of two Girella species, thus increasing the efficiency and quality of Girella species stock management and forensic identification to prevent species misidentification.

Funder

Korea Institute of Marine Science and Technology Promotion funded by the Ministry of Oceans and Fisheries

National Institute of Fisheries Science, Ministry of Oceans and Fisheries, Korea

Publisher

MDPI AG

Subject

Ecology,Aquatic Science,Ecology, Evolution, Behavior and Systematics

Reference18 articles.

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2. Comparison of Morphological Characteristics between Smallscale Blackfish, Girella leonine and Largescale Blackfish, G. punctata;Lim;J. Fish. Mar. Sci. Educ.,2016

3. Evolutionary trend in feeding habits of Girella (Perciformes: Girellidae);Yagishita;Ichthyol. Res.,2003

4. Revision of the genus Girella (Girellidae) from East Asia;Yagishita;Ichthyol. Res.,2000

5. Identification of Girella punctate and G. leonine by PCR-RFLP analysis;Itoi;J. Mar. Sci.,2007

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