1996
DOI: 10.1111/j.0022-3646.1996.00424.x
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ANALYSIS OF ALEXANDRIUM (DINOPHYCEAE) SPECIES USING SEQUENCES OF THE 5.8S RIBOSOMAL DNA AND INTERNAL TRANSCRIBED SPACER REGIONS1

Abstract: The 5.8S ribosomal RNA gene (rDNA) and flanking internal transcribed spacers 1 and 2 (ITS1 and ITS2) from 7 isolates of Alexandrium catenella (Wedon et Kofoid) Taylor, 13 isolates of A. tamarense (Lebour) Balech, 2 isolates of A. affine (Fukuyo et Inoue) Balech, and single isolates of A. fundyense Balech, A. insuetum Balech, and A. pseudogonyaulax (Biecheler) Horiguchi ex Yuki et Fukuyo comb. nov. from Japan, Thailand, and the United States were amplified using the polymerase chain reaction (PCR), sequenced, a… Show more

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Cited by 190 publications
(149 citation statements)
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“…Lysis was made using warm lysis buffer (65 8C), cells were transferred to a suspension of glass beads and disrupted and homegenised by reciprocal shaking at maximum speed (6.5 m s À1 ) in a FastPrep instrument (Thermo Savant, Illkirch, France), 4 mL of RNAse was added, and elution was made in 50 mL of elution buffer. Polymerase chain reaction (PCR) for large subunit ribosomal DNA (LSU rDNA) was performed using primers D1 C (5 0 -ACCCGCTGAATTTAAGCATA-3 0 ) and D2R (5 0 -CCTTGGTCCGTGTTTCAAGA-3 0 ) (Scholin et al, 1994), and PCR for internal transcribed spacer ribosomal DNA (ITS rDNA) was performed using primers ITSa (5 0 -CCAAGCTTCTAGATCGTAACAAG-G(ACT)TCCGTAGGT-3 0 ) and ITSb (5 0 -CCTGCAGTCGACA(GT)ATGCT-TAA(AG)TTCAGC(AG)GG-3 0 ) (Adachi et al, 1996). Genomic DNA was amplified in a 20 mL PCR reaction containing 16.3 mL of milliQ water, 2.0 mL of 10Â HotMaster Taq Buffer (Eppendorf), which included MgCl 2 , 0.2 mL of each primer (10 mM), 0.2 mL of dNTP (10 mM), 0.1 ml HotMaster Taq polymerase (Eppendorf), and 10 ng of DNA mL À1 .…”
Section: Molecular Phylogeny 251 Dna Extraction and Sequencingmentioning
confidence: 99%
“…Lysis was made using warm lysis buffer (65 8C), cells were transferred to a suspension of glass beads and disrupted and homegenised by reciprocal shaking at maximum speed (6.5 m s À1 ) in a FastPrep instrument (Thermo Savant, Illkirch, France), 4 mL of RNAse was added, and elution was made in 50 mL of elution buffer. Polymerase chain reaction (PCR) for large subunit ribosomal DNA (LSU rDNA) was performed using primers D1 C (5 0 -ACCCGCTGAATTTAAGCATA-3 0 ) and D2R (5 0 -CCTTGGTCCGTGTTTCAAGA-3 0 ) (Scholin et al, 1994), and PCR for internal transcribed spacer ribosomal DNA (ITS rDNA) was performed using primers ITSa (5 0 -CCAAGCTTCTAGATCGTAACAAG-G(ACT)TCCGTAGGT-3 0 ) and ITSb (5 0 -CCTGCAGTCGACA(GT)ATGCT-TAA(AG)TTCAGC(AG)GG-3 0 ) (Adachi et al, 1996). Genomic DNA was amplified in a 20 mL PCR reaction containing 16.3 mL of milliQ water, 2.0 mL of 10Â HotMaster Taq Buffer (Eppendorf), which included MgCl 2 , 0.2 mL of each primer (10 mM), 0.2 mL of dNTP (10 mM), 0.1 ml HotMaster Taq polymerase (Eppendorf), and 10 ng of DNA mL À1 .…”
Section: Molecular Phylogeny 251 Dna Extraction and Sequencingmentioning
confidence: 99%
“…The LSU primers were DIR-F (5′-ACCCGCTGAA TTTAAGCATA-3′) and Dir-2C (5′-CCTTGGTCCGTGTTT CAAGA-3′), according to Scholin et al (1994). The PCR steps were a hold at 94°C for 9 min, followed by 20 cycles of 94°C for 30 s, 55°C for 30 s and 72°C for 9 m. For ITS, we used ITS A (5′-CCAAGCTTCTAGATCGTAACAAGGHT CCGTAGGT-3′) and ITS B (5′-CCTGCAGTCGACAKA TGCTTAARTTCAGCRGG-3′) (Adachi et al, 1996), with PCR steps comprising a hold at 94°C for 5 min, followed by 35 cycles of 94°C for 20 s, 57°C for 10 s and 70°C for 5 min. The primers for rbcL were 130F (5′-AACWACWACTTGG ATTTGGAA-3′) and 1600R (5′-GCATGAATATGMTG WACCAT-3′) (Yoon et al, 2002), with PCR steps comprising a hold at 94°C for 2 min, followed by 39 cycles of 94°C for 20 s, 46°C for 30 s and 70°C for 5 min.…”
Section: Culturesmentioning
confidence: 99%
“…A partial LSU rDNA sequence, including the D1 and D2 domains, was amplified by polymerase chain reaction (PCR) using primers D1R and D2C (Scholin et al 1994). The total ITS1-5.8S-ITS2 was amplified using ITSA and ITSB primers (Adachi et al 1996). The PCR protocol was as follows: 94 8C for 3.5 min; followed by 35 cycles of 94 8C for 50 s, 45 8C for 50 s, 72 8C for 80 s; plus a final extension of 72 8C for 10 min.…”
Section: Molecular Analysismentioning
confidence: 99%