Abstract
Nucleotide sequences in internal transcribed spacer (ITS)-1 region derived from dried nori products produced in Japan, China, and the Republic of Korea were compared. Thalli contained in the Japanese products were genetically homogenous, and their nucleotide sequences in ITS-1 were identical to those of the reference strains of Pyropia yezoensis f. narawaensis. In Chinese products, the thalli were related to P. yezoensis strain Minomiasakusa. In contrast, the thalli in the Korean products were genetically heterogeneous, and several different P. yezoensis strains and other Pyropia spp. were used for dried nori products. In some thalli produced in both China and Korea, the DNA sequences of the ITS-1 region were identical with that of Japan, suggesting that the cultivar strains might have been transplanted from Japan to China in recent years. The 432-bp-long nucleotide sequences in the ITS-1 region of thalli derived from Japanese origin were cleaved to two restriction fragments at 154 and 278 bp by cleavage of PCR-amplified products using MspI. Conversely, almost all of the corresponding sequences derived from China and Korea were lacking MspI or other restriction patterns, except for nori products from some areas that cultivate a closely related strain to the Japanese cultivar.
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Introduction
“Nori” (edible seaweed, Pyropia yezoensis) is one of the most important aquaculture species in Japan [1]. Nori is cultivated on the surface of the sea; the thalli are cut, dried, pressed in a sheet, and then distributed as dried products [1]. Seaweed farms are distributed along the coastal area from southern to northern Japan [1]. Nori is also farmed in China and the Republic of Korea with the help of technological know-how and the transplantation of some strains of P. yezoensis from Japan [1]. P. yezoensis f. narawaensis, which has been established by selective breeding from cultivated populations, now dominates farms in Japan [2, 3].
Labeling is necessary for fresh marine products and processed foods to assist consumers in selecting foods according to the Law on Standardization and Proper Labeling of Agricultural and Forestry Products [Japan Agricultural Standard (JAS) Law]. For imported marine products, country-of-origin food labeling is required in the Japanese market. In addition to the import of nori products from the Republic of Korea, an import quota on nori products from China has been in place since 2005, and dried nori products are now imported from both countries. Therefore, biochemical and genetic techniques for origin identification are needed for dried nori products to certify whether country-of-origin food labeling is correct.
Molecular identification techniques of Pyropia spp. and P. yezoensis strains have been developed previously. DNA fingerprinting and PCR-based restriction fragment length polymorphism (RFLP) analysis have been conducted using small subunit ribosomal RNA [4], internal transcribed spacer region (ITS) [2, 5–8], plastid ribulose bisphosphate carboxylase/oxygenase gene (RuBisCo) [6–8], and actin-related protein 4 gene [9]. Park et al. [10] reported genetic polymorphism within wild-collected P. yezoensis from Japan and Korea. In 2011, the red algal order Bangiales has been revised based on combined analyses of the nuclear SSU rRNA gene and the RuBisCo L gene [11]. Mitochondrial DNA was also used for the discrimination of 18 Japanese Porphyra and Pyropia species [12]. From these previous studies, Kunimoto et al. [2] and Niwa et al. [8] reported diverse nucleotide sequences in the ITS region among P. yezoensis wild-collected and culture strains. Therefore, to develop origin identification techniques for dried nori products, nucleotide sequences in the ITS region are required to determine and compare the thalli DNA extracted from dried nori products produced in Japan, Korea, and China. In Pyropia aquaculture, a mixed culture of several distinct cultivated strains is used for seed production to promote enhanced adaptation to different environmental situations. In addition, natural conchospores may be contaminated by cultivation nets in the sea. Therefore, a possibility existed that distinct DNA sequences derived from several cultured and wild strains might be detected in a single sheet of dried nori product. Thus, we isolated each thallus piece from dried nori products, and carefully determined its nucleotide sequence in the ITS region.
This study focused on differences between the nucleotide sequences in the ITS-1 region from the thalli in dried nori products produced in Japan, Korea, and China. According to the nucleotide differences between Japanese and the other two countries, we identified marker nucleotide sequences specific to dried nori products produced in Japan, Korea or China. In addition, we developed PCR–RFLP analysis methods for discriminating between the nori products produced in Japan, and those imported from Korea or China.
Materials and methods
Materials
Dried nori products were obtained from Japan, China, and Korea between 2006 and 2008. Nori samples were stored with desiccant at −20 °C until use.
DNA extraction, PCR amplification, and sequencing
Nori sheets were cut into small pieces, and individual pieces were swollen and dissociated in distilled water. Each piece of thalli was put into a 1.5-ml tube and then stored at −20 °C until use. From 2 to 16 pieces were sampled from each nori sheet. One piece of thallus was thawed and ground with a mortar and pestle. Total DNA was extracted from the ground sample using the Illustra DNA Extraction Kit Phytopure (GE Healthcare, Wauwatosa, WI, USA) or DNeasy Plant Mini Kit (Qiagen, Hilden, Germany) according to the manufacturer’s protocol. The nuclear ITS-1 region was amplified using Premix Taq (ExTaq Version: Takara Bio, Ohtsu, Japan) and 0.2 μM of the forward primer (CCGTAGGTGAACCTGCGGAAGGATCAT) and the reverse primer (CAAGATATCCACCGCTAAGAGTTGTAT). The PCR program was for 120 s at 96 °C, followed by 30–40 cycles of 15 s at 96 °C, 15 s at 55 °C, and 15 s at 72 °C, and finally 180 s at 72 °C. The products were treated with ExoSAP-IT (GE Healthcare) and then sequenced. The plastid RuBisCo and its spacer region were amplified with Premix Taq using 0.2 μM of the forward primer (ATGTCTCAATCCGTAGAATCACG) and the reverse primer (TTAATATCTAGCTCCTTCAGGC) based on the small subunit ribosomal RNA gene and 5.8S ribosomal RNA gene, which are both highly conserved among Pyropia species. The PCR program was for 120 s at 96 °C, followed by 30–40 cycles of 15 s at 96 °C, 15 s at 55 °C, and 60 s at 72 °C, and finally 180 s at 72 °C. The products were treated with ExoSAP-IT and then sequenced. The products were sequenced using an ABI PRISM 3100 Genetic Analyzer or ABI PRISM 3130xl Genetic Analyzer (Life Technologies Corporation, Carlsbad, CA, USA) with ABI PRISM BigDye Terminator v3.1. The nucleotide sequences in the ITS-1 region and the RubisCo gene in various Pyropia species were aligned using the CLUSTALW program [13] on the web site of the DNA Database Bank of Japan, and a phylogenetic tree was designed using the Treeview ppc version 1.6.6 program [14]. The nucleotide sequences determined in this study were deposited in the DDBJ/EMBL/GenBank DNA Database (accession numbers AB818905–AB818921).
Restriction fragment length polymorphism
Amplified PCR products of the ITS-1 region were digested with MspI restriction enzyme (New England Biolabs Japan, Tokyo, Japan). A reaction mixture of 10 μl containing from 2 to 3 μl of PCR product, 5 units of MspI, 1 μl of restriction enzyme buffer, and distilled water was incubated at 37 °C for at least 3 h. The reaction mixture was separated in a 3 % agarose gel containing ethidium bromide and photographed under ultraviolet light.
Results
Comparison of nucleotide sequences in the ITS-1 region of the dried nori products
Total DNA was extracted from the dried nori products produced in Japan, China, and Korea, and PCR amplification products were of similar size, approximately 430 bp long, except for some pieces from Korea (Fig. 1, lanes 1–6). The nucleotide sequences of the partial PCR fragment in the approximately 430-bp-long ITS-1 region were determined to identify DNA polymorphism in Pyropia species and P. yezoensis strains contained in the nori products (Fig. 2).
Almost all of the 343-bp-long partial nucleotide sequences in the ITS-1 region of 90 pieces of thalli derived from Japanese origin in the present study were identical to those of P. yezoensis f. narawaensis. This genotype was tentatively named “Japan_Sub01” in Table 1. In this sequence, we found an MspI gene site at 126 bp as shown in Fig. 2, and two restriction fragments at 154 and 278 bp by cleavage of PCR-amplified products using MspI restriction enzymes. Therefore, we found close relationships between most of the cultured nori strains, except for two samples that were considered to be a wild strain (“Japan_Sub02”). The Japan_Sub02 genotype was detected in only one piece of thallus, as compared with 15 pieces having the genotype Japan_Sub01.
The dried nori products produced in China had two specific genotypes denoted “China_Sub01” and “China_Sub02” marked by a single nucleotide deletion of the nucleotide sequence of the partial ITS-1 region of the P. yezoensis strain Minomiasakusa [2]. The China_Sub02 genotype had a single nucleotide insertion in the region of the 5.8S rRNA gene in the 426-bp long partial ITS-1 sequence in the China_Sub01 genotype. Among 160 pieces of thalli samples prepared from 54 dried nori products in China, 151 pieces had these Chinese-specific genotypes (Table 2). The remaining nine pieces had nucleotide sequences that were identical to Japan_Sub02.
The ITS-1 region was determined in 263 pieces of thalli samples prepared from 34 dried nori products produced in Korea. These 263 nucleotide sequences were classified into 11 genotypes of P. yezoensis strains: Japan_Sub01, China_Sub01&02, Korea_SubA01, Korea_SubA02, Korea_SubA03, Korea_SubA04, Korea_SubB01, Korea_SubB02, Korea_SubB03, and two genotypes of Pyropia sp. NRIFS-1 and NRIFS-2 that were not P. yezoensis (Table 3). The genotype Korea_SubA01 was identical to the nucleotide sequences of P. yezoensis wild strains NS003 and NS004 isolated from natural seeding on the southwest coast of Korea (accession numbers DQ227869 and DQ227870, respectively). Nucleotide sequences in the ITS-1 region of the genotypes Korea_SubB01, Korea_SubB02, and Korea_SubB03 were identical to those of P. yezoensis strains NS005 (accession no. DQ227871), NS002 (accession no. DQ227868), and NS001 (accession no. DQ227867) isolated from the natural seeds of wild strains in Korea, respectively. Thalli whose ITS-1 region’s DNA sequences were identical to those in Japan (Japan_Sub01) or China (China_Sub01) were also detected (Table 3). These genotypes, China_Sub01-02, Korea_SubA01-A04, and Korea_SubB01-B03, closely resembled P. yezoensis strain Minomiasakusa, rather than resembling P. yezoensis strain f. narawaensis, in phylogenetic analysis (Fig. 3). In addition, two Pyropia spp. whose DNA sequences of the ITS-1 region completely differed from those of P. yezoensis strains were detected only in the dried nori products from Korea (Table 3). Among 263 pieces of thalli in the Korean products, 50 pieces contained the 348-bp-long segment of the ITS-1 region (Pyropia sp. NRIFS-1) and two pieces contained the approximately 350-bp-long segment of the ITS-1 region (Pyropia sp. NRIFS-2), whose nucleotide sequences differed from those of P. yezoensis. However, we could not determine these nucleotide sequences in the ITS-1 region of Pyropia sp. NRIFS-1 and NRIFS-2 because of highly repetitive nucleotide sequences. We also analyzed the nucleotide sequences of plastid RuBisCo genes. Phylogenetic analysis based on the nucleotide sequences of the RuBisCo gene in the Pyropia genus showed that these sequences in Pyropia sp. NRIFS-1 and Pyropia sp. NRIFS-2 were included in a cluster of Pyropia spp. The nucleotide sequence for Pyropia sp. NRIFS-1 was closely related to those of P. dentata and P. haitanensis (Fig. 4), and identical by 95 and 94 %, respectively. The nucleotide sequence of Pyropia sp. NRIFS-2 was closely related to P. katadae and P. tenuipedalis (Fig. 4), and was identical by 96 and 96 %, respectively. By additional BLAST analyses using the RuBisCo L gene, the nucleotide sequence of Pyropia sp. NRIFS-1 was very similar to that of P. seriata that was isolated in Kumamoto, Japan (HQ687533) [11] with 99.8 % nucleotide identity. The nucleotide sequence of Pyropia sp. NRIFS-2 in the RuBisCo L gene was identical to those of P. kuniedae (HQ728200) and P. pulchella (GU046419) [11].
In contrast, nine dried nori products produced in Gimhae and Pusan (Table 3) contained only the thalli of the strain whose DNA sequence was identical with that from Japan (Japan_Sub01).
RFLP analysis
The nucleotide sequences showed two distinct RFLP patterns using MspI that differed by origin. The genotype Japan_Sub01 contained a 432-bp-long DNA sequence with an MspI site, resulting in 154 and 278-bp fragments isolated by RFLP (Fig. 1, lane 7). Other genotypes such as Japan_Sub02, China_Sub01, Korea_SubA01, Korea_SubA02, and Korea_SubA03, found in most of the dried nori products produced in China and Korea, contained a DNA sequence with no MspI site (Fig. 1, lanes 8–10). Other genotypes, such as Korea_SubB01, Korea_SubB02, and Korea_SubB03, also contained a 426-bp-long DNA sequence with an MspI site (Fig. 1, lane 11). In 116 dried nori products from Japan, PCR products with no MspI site were detected in only two pieces of thalli from over 1,200 samples.
Discussion
The nucleotide sequences of the ITS region extracted from the thalli of dried nori products from Japan, China, and Korea were compared to discriminate between countries-of-origin for the food labeling of dried nori products. Differences in the nucleotide sequences of dried nori products from Japan, China, and Korea were identified, and genetic variation in P. yezoensis and other related species was characterized in these different country-of-origin products.
In Japanese products, the genetic variation of P. yezoensis was very low, and the nucleotide sequences in the ITS region of almost all products were identical to the genotype Japan_Sub01, which corresponded to the reference strains of P. yezoensis f. narawaensis (i.e., U-51, Saga-5, Sasiki, Fukuoka-1, Ariake-1, and Saga103) [5, 8]. The two exceptional cases in which we detected the genotype Japan_Sub02 may have been due to contamination by wild strains in the aquaculture field. In recent years, specific strains have been obtained by the selective breeding of P. yezoensis f. narawaensis in Japanese institutes and have been applied in commercial production [1–3]. Therefore, genetic homogeneity may be increased by the selective breeding of nori cultivar strains. In Chinese products, the cultivar strain that was closely related to the P. yezoensis strain Minomiasakusa, was detected in 41 of the 45 products used in this study. The Minomiasakusa strain was established from a wild strain in 1979 by a Japanese company (http://www.hinsyu.maff.go.jp/tokei/contents/14_2012kaiso.pdf). The genotypes China_Sub01 and China_Sub02 may have been derived from the Minomiasakusa strain and transplanted from Japan. On the other hand, three products produced in Qingdao had the genotype Japan_Sub01 identical to that of P. yezoensis f. narawaensis, suggesting that cultivar strains may have been transplanted from Japan to China in recent years.
In the Korean products, many genetically distinct genotypes of strains were detected. Four genotypes, Korea_SubA01, SubB01, SubB02, and SubB03, were identical to known cultivar strains of P. yezoensis isolated from natural seeds of Korea’s southwest coast, according to the DNA database. These genotypes have never been found in Japanese products or cultivar and wild strains, suggesting they were transplanted from Japan in earlier years. Based on the partial nucleotide sequences in the RuBisCo L gene, the sequence of Pyropia sp. NRIFS-1 was closely related to that of P. seriata [11], and that of Pyropia sp. NRIFS-2 was identical to those of P. kuniedae and P. pulchella [11]. These were used in the Korean products, indicating that Pyropia species, other than P. yezoensis, are also cultured for the production of dried nori products. In addition, the genotype Japan_Sub01 of P. yezoensis was also used in the Korean products, suggesting that this genotype was transplanted from Japan in recent years. Recent studies characterized the phylogenetic relationship in Pyropia spp. by analyses of mitochondrial and plastid DNA [11, 12]. Therefore, mitochondrial and plastid DNA analysis may also be useful for species and origin identification of the Korean dried nori products.
This study showed that RFLP analysis of the ITS region by cleavage with MspI is useful for the discrimination of Japanese domestic dried nori products versus those imported from China and Korea. However, some exceptional samples from the Chinese or Korean products showed similar RFLP patterns to Japanese products. In such cases, multiple trace elemental analysis can support RFLP analysis by MspI cleavage [15].
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Acknowledgments
The authors are grateful to Dr. Masahiko Kunimoto for helpful suggestions. We thank the Japan Fisheries Cooperatives, Japan Nori Association, National Federation of Nori and Clams Fisheries Cooperatives, Okayama Prefectural Fisheries Experiment Station, Saga Prefectural Ariake Fisheries Research and Development Center, Seikai National Fisheries Institute, Takaokaya Inc., and Fujimori-Shoten for providing the seaweed samples. This work was supported by funding from the Fisheries Agency, Japan.
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Touhata, K., Namikoshi, A., Suzuki, T. et al. Origin identification of dried seaweed product “nori” by PCR–RFLP analysis of Pyropia yezoensis in the internal transcribed spacer ITS-1 region. Fish Sci 79, 865–875 (2013). https://doi.org/10.1007/s12562-013-0661-2
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DOI: https://doi.org/10.1007/s12562-013-0661-2