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  • A chimeric protein of alumi...
    Sasaki, Takayuki; Tsuchiya, Yoshiyuki; Ariyoshi, Michiyo; Ryan, Peter R.; Yamamoto, Yoko

    Biochimica et biophysica acta, July 2016, 2016-Jul, 2016-07-00, Letnik: 1858, Številka: 7
    Journal Article

    TaALMT1 from wheat (Triticum aestivum) and AtALMT1 from Arabidopsis thaliana encode aluminum (Al)-activated malate transporters, which confer acid–soil tolerance by releasing malate from roots. Chimeric proteins from TaALMT1 and AtALMT1 (Ta::At, At::Ta) were previously analyzed in Xenopus laevis oocytes. Those studies showed that Al could activate malate efflux from the Ta::At chimera but not from At::Ta. Here, functions of TaALMT1, AtALMT1 and the chimeric protein Ta::At were compared in cultured tobacco BY-2 cells. We focused on the sensitivity and specificity of their activation by trivalent cations. The activation of malate efflux by Al was at least two-fold greater in the chimera than the native proteins. All proteins were also activated by lanthanides (erbium, ytterbium, gadolinium, and lanthanum), but the chimera again released more malate than TaALMT1 or AtALMT1. In Xenopus oocytes, Al, ytterbium, and erbium activated inward currents from the native TaALMT1 and the chimeric protein, but gadolinium only activated currents from the chimera. Lanthanum inhibited currents from both proteins. These results demonstrated that function of the chimera protein was altered compared to the native proteins and was more responsive to a range of trivalent cations when expressed in plant cells. Display omitted •Malate efflux activated by trivalent cations was compared between Ta::At chimera and native ALMT proteins.•Malate efflux activated by Al and lanthanides was greater from the chimera than the native proteins in BY-2 cells.•Malate efflux from the chimera was activated by these lanthanides except for La3+ in Xenopus oocytes.•Thus the chimeric protein shows enhanced response to various trivalent cations in plant–cell system.