Plant Nucleotide Metabolism. Hiroshi Ashihara

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Название Plant Nucleotide Metabolism
Автор произведения Hiroshi Ashihara
Жанр Биология
Серия
Издательство Биология
Год выпуска 0
isbn 9781119476078



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Xanthosine* → Xanthine* + Ribose (9) 8.7 29.1

      Enzyme activity is expressed as pkat mg−1 protein; a) no activity detected.

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      Since activity of adenosine nucleosidase (EC 3.2.2.7), inosine/guanosine nucleosidase (EC 3.2.2.2), and/or purine nucleosidase (EC 3.2.2.1) occur in potato tubers and tea leaves (Table 5.1), simple hydrolysis of purine nucleosides to purine bases would appear to be the main route in plants. However, purine base formation from purine nucleosides catalysed by purine phosphorylase, or by the reverse reaction of phosphoribosyltransferases, appears not to participate in this hydrolysis in plants. Properties of nucleosidases are described with the interconversion of purines in Chapter 6.

      5.3.1 Adenine Phosphoribosyltransferase

      The Arabidopsis genome has five APRT sequences (Table 5.2), three of which, APT1, APT2, and APT3, have been cloned, overexpressed, and their catalytic properties characterized (Moffatt et al. 1992). All three isozymes bind adenine (Km: <3 μM). One of the isoenzymes (APT1) is 40–80 times more efficient, judged by the Vmax/Km ratio, in metabolizing adenine than the other isozymes. Since none of the predicted amino acid sequences for the adenine phosphoribosyltransferases (APTs) of A. thaliana appear to contain transit signalling peptides, APTs are assumed to be located in the cytosol. However, the findings of Zybailov et al. (2008) suggest that an isoform of APT1 has a transit peptide for chloroplasts. Traditional biochemical analysis indicates that in addition to the cytosol, APRT also occurs in plastids and mitochondria in some plants, (see Ashihara et al. 2018). Biochemical analysis indicates that large quantities of APRT activity are located in cytosol, but substantial amounts are also found in chloroplasts of spinach (Ashihara and Ukaji 1985) and tea leaves (Koshiishi et al. 2001), as well as mitochondria of Catharanthus roseus cells (Hirose and Ashihara 1982) and tubers of Jerusalem artichoke (Helianthus tuberosus) (Le Floc'h and Lafleuriel 1983). Although the occurrence of APRT in mitochondria has not yet been confirmed at the molecular level, purified intact mitochondria from C. roseus are capable of synthesizing adenine nucleotides from 14C-labelled adenine (Ukaji et al. 1986).

      5.3.2 Hypoxanthine/Guanine Phosphoribosyltransferase

      HGPRT (IMP/GMP): diphosphate phospho-D-ribosyltransferase, EC 2.4.2.8) catalyses the formation of IMP (or GMP) from inosine (or guanine) and PRPP. Although HGPRT activity is generally high in mammalian tissues (Adams and Harkness 1976), in plants it is usually much lower than that of APRT (Table 5.1).

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Km values (μM)
Enzyme Enzyme source Isozyme Optimum pH A PRPP tZ iP BA Gene TAIR locus Reference
APRT 5.5–6.5 5.5 64