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當(dāng)前位置 > 首頁 > 技術(shù)文章 > 異鈣調(diào)素結(jié)合在質(zhì)膜胞外位點(diǎn)上并導(dǎo)致胞內(nèi)鈣離子水平上升

異鈣調(diào)素結(jié)合在質(zhì)膜胞外位點(diǎn)上并導(dǎo)致胞內(nèi)鈣離子水平上升

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                     鈣調(diào)素的研究被Nature China評為一周研究亮點(diǎn)
            異鈣調(diào)素結(jié)合在質(zhì)膜胞外位點(diǎn)上并導(dǎo)致胞內(nèi)鈣離子水平上升
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上圖:百合花粉CaM的定位以及原生質(zhì)體質(zhì)膜Ca2+

鈣調(diào)蛋白(CaM)是一種高保守性的細(xì)胞內(nèi)鈣離子感應(yīng)器。在植物中,胞外CaM也作為一個(gè)多肽信號(hào)影響許多生理功能,但是其在細(xì)胞質(zhì)外的結(jié)合位點(diǎn)至今仍存在爭議。

2009年5月,中科院植物所林金星研究組在《JBC》上發(fā)表文章,研究人員利用CaM交聯(lián)QD系統(tǒng)對植物細(xì)胞表面CaM結(jié)合位點(diǎn)進(jìn)行單分子水平檢測,發(fā)現(xiàn)QD-CaM能選擇性的結(jié)合在質(zhì)膜外空間,并且通過高分辨率透射電子顯微鏡進(jìn)行了進(jìn)一步定位,證實(shí)了胞外CaM結(jié)合位點(diǎn)確實(shí)存在于植物細(xì)胞膜表面,但在植物細(xì)胞壁上卻沒有CaM結(jié)合位點(diǎn)。此研究為鈉米技術(shù)在植物細(xì)胞研究上的應(yīng)用提供了有力的證據(jù)。此外,研究人員還利用顯微注射、FRET以及非損傷微測(SIET)等技術(shù)證明了胞外CaM在與其胞外結(jié)合為點(diǎn)結(jié)合后,可以引起胞內(nèi)第二信使Ca2+信號(hào)的增強(qiáng),這些發(fā)現(xiàn)說明了植物胞外CaM可以通過介導(dǎo)跨膜信號(hào)而發(fā)揮其信號(hào)肽的功能。

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關(guān)鍵詞:鈣調(diào)素(Calmodulin, CaM);離子選擇性電極(Ion-selective microelectrodes);質(zhì)膜(Plasma membrane)
參考文獻(xiàn):Wang et al. J. Biol. Chem..2009, 284: 12000-12007
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Abstract
Calmodulin (CaM) is a highly conserved intracellular calcium sensor. In plants, CaM also appears to be present in the apoplasm, and application of exogenousCaMhas been shown to influence a number of physiological functions as a polypeptide signal; however, the existence and localization of its corresponding apoplasmic binding sites remain controversial. To identify the site(s) of action, a CaM-conjugated quantum dot (QD) system was employed for single molecule level detection at the surface of plant cells. Using this approach, we show that QD-CaM binds selectively to sites on the outer surface of the plasma membrane, which was further confirmed by high resolution transmission electron microscopy. Measurements of Ca2+ fluxes across the plasma membrane, using ion-selective microelectrodes, demonstrated that exogenous CaM induces a net influx into protoplasts. Consistent with these flux studies, calcium-green-dextran and FRET experiments confirmed that applied CaM/QD-CaM elicited an increase in cytoplasmic Ca2+ levels. These results support the hypothesis that apoplasmic CaMcan act as a signaling agent. These findings are discussed in terms of CaM acting as an apoplasmic peptide ligand to mediate transmembrane signaling in the plant kingdom.
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