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Volumn 274, Issue 5288, 1996, Pages 801-804

Visual pigment gene structure and the severity of color vision defects

Author keywords

[No Author keywords available]

Indexed keywords

VISUAL PIGMENT;

EID: 0029858647     PISSN: 00368075     EISSN: None     Source Type: Journal    
DOI: 10.1126/science.274.5288.801     Document Type: Article
Times cited : (98)

References (31)
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    • J. Neitz and G. H. Jacobs. Nature 323. 623 (1986); Vision Res. 30, 621 (1990)
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    • Neitz, J.1    Jacobs, G.H.2
  • 2
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    • J. Neitz and G. H. Jacobs. Nature 323. 623 (1986); Vision Res. 30, 621 (1990)
    • (1990) Vision Res. , vol.30 , pp. 621
  • 4
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    • note
    • The degree of color vision defect can be expressed quantitatively from measurements of the colors in the designs as specified by their coordinates, in this case in units of the Commission International de l'Éclairage (CIE) u′ v′ diagram [following (4)]. For normal color vision, this represents an approximation of a two-dimensional color diagram in which equal distances in different locations correspond to equal perceptual differences. Thus, the extent of the defect can be expressed numerically as the distance (D) in the color diagram that must differentiate the symbol from its background before the person can interpret it correctly.
  • 11
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    • J. Pokorny and V. C. Smith, J. Opt Soc. Am. 67, 1196 (1977); Color Res. Appl. 7, 159 (1982); P. De-Marco, J. Pokorny, V. C. Smith, J. Opt. Soc. Am. A 9, 1465 (1992); T. P. Piantanida, Am. J. Optom. Physiol. Opt. 53, 647 (1976).
    • (1977) J. Opt Soc. Am. , vol.67 , pp. 1196
    • Pokorny, J.1    Smith, V.C.2
  • 12
    • 0020141020 scopus 로고
    • J. Pokorny and V. C. Smith, J. Opt Soc. Am. 67, 1196 (1977); Color Res. Appl. 7, 159 (1982); P. De-Marco, J. Pokorny, V. C. Smith, J. Opt. Soc. Am. A 9, 1465 (1992); T. P. Piantanida, Am. J. Optom. Physiol. Opt. 53, 647 (1976).
    • (1982) Color Res. Appl. , vol.7 , pp. 159
  • 13
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    • J. Pokorny and V. C. Smith, J. Opt Soc. Am. 67, 1196 (1977); Color Res. Appl. 7, 159 (1982); P. De-Marco, J. Pokorny, V. C. Smith, J. Opt. Soc. Am. A 9, 1465 (1992); T. P. Piantanida, Am. J. Optom. Physiol. Opt. 53, 647 (1976).
    • (1992) J. Opt. Soc. Am. A , vol.9 , pp. 1465
    • De-Marco, P.1    Pokorny, J.2    Smith, V.C.3
  • 14
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    • J. Pokorny and V. C. Smith, J. Opt Soc. Am. 67, 1196 (1977); Color Res. Appl. 7, 159 (1982); P. De-Marco, J. Pokorny, V. C. Smith, J. Opt. Soc. Am. A 9, 1465 (1992); T. P. Piantanida, Am. J. Optom. Physiol. Opt. 53, 647 (1976).
    • (1976) Am. J. Optom. Physiol. Opt. , vol.53 , pp. 647
    • Piantanida, T.P.1
  • 18
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    • T. Chan, M. Lee, T. P. Sakmar, J. Biol. Chem. 267, 9478 (1992); A. J. Williams, D, M Hunt, J, K. Bowmaker, J. D. Mollon, EMBO J. 11. 2039 (1992).
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    • Chan, T.1    Lee, M.2    Sakmar, T.P.3
  • 22
    • 10544225065 scopus 로고    scopus 로고
    • note
    • The Expand Long Template PCR System (Boehringer Mannheim) was used exactly as recommended by the manufacturer to do long PCR. The first gene in the array was amplified in long PCR with primers 5′-GAGGCGAGGCTACGGAGT and 5′-ACGGTATTTTGAGTGGATCTGCT, which correspond to sequences 862 base pairs (bp) upstream of the first exon of the first gene (23) and to the 3′ end of intron 5 (8), respectively. The PCR product served as a template to amplify exons 2, 3, 4, and 5 as described previously (2, 8, 24).
  • 23
    • 10544248712 scopus 로고    scopus 로고
    • note
    • Restriction analysis was done on exons 3, 4, and 5 from the first gene and on exons 3 and 4 from downstream L genes. The presence of an Rsa I site in exon 5 from the first gene from each male identified it as a L pigment gene (8). Whether exon 3 contains a Bso Fl restriction site or not indicates whether codon 180 specifies alanine or serine, respectively (24). A Dde l site is found in exon 4 only when serine is specified by codon 233. and this was used to deduce whether the first gene or the downstream L genes were M4L5 hybrids. The results of the restriction analyses were confirmed by direct sequence analysis (24), which was also used to determine whether the sequence of exon 2 differed among the L pigment genes in individual men.
  • 24
    • 10544247886 scopus 로고    scopus 로고
    • note
    • For men whose L pigment genes did not differ in exon 4 (Fig. 1C), all L genes except the first gene in the array were amplified by long-PCR (17) with primers 5′-TTAGTCAGGCTGGTCGGGAACT and 5′-CATGATGATAGCGAGTGGGATG, which correspond to sequences 465 bp upstream of the first exon of all genes in the array except the first one (5), and to L gene-specific exon 4 sequences (24), respectively. For men whose L genes differed in exon 4 (Fig. 1C), no PCR product was obtained with this primer pair, presumably because their downstream L genes were hybrid genes with an M gene exon 4 sequence. For these men, downstream L pigment genes were selectively amplified by long PCR (17) with the use of an exon 2 primer (5′-CCTTCGAAGGCCCGAATTA) paired with a L gene-specific exon 5 primer (24), The PCR product was used to amplify only the downstream L pigment genes with the use of the same exon 2 primer and an M gene-specific exon 4 primer (24).
  • 27
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    • An exception, however, is a model, progressive for its time, forwarded by M. Alpern and J. Moeller who proposed variation in normal L pigments [J. Physiol. (London) 266, 647 (1977)].
    • (1977) J. Physiol. (London) , vol.266 , pp. 647
    • Alpern, M.1    Moeller, J.2
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    • Y. Wang et al, Neuron 9, 429 (1992).
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  • 31
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    • note
    • We thank P. Summerfelt for help in preparing the manuscript and G. H. Jacobs for his many helpful suggestions and comments. Supported by NIH grants EY09303, EY09620, and EY01931, and by Research to Prevent Blindness James. S. Adams Scholar Award to M.N.


* 이 정보는 Elsevier사의 SCOPUS DB에서 KISTI가 분석하여 추출한 것입니다.