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在正常发育的葡萄(Vitis vinifera L.)浆果整个发育过程中,膜完整性和细胞活力得到显著维持的证据。

Evidence for substantial maintenance of membrane integrity and cell viability in normally developing grape (Vitis vinifera L.) berries throughout development.

作者信息

Krasnow Mark, Matthews Mark, Shackel Ken

机构信息

University of California, Davis, One Shields Avenue, Davis, CA 95616, USA.

出版信息

J Exp Bot. 2008;59(4):849-59. doi: 10.1093/jxb/erm372. Epub 2008 Feb 13.

Abstract

Fluorescein diacetate (FDA) was used as a vital stain to assay membrane integrity (cell viability) in mesocarp tissue of the developing grape (Vitis vinifera L.) berry in order to test the hypothesis that there is a substantial loss of compartmentation in these cells during ripening. This technique was also used to determine whether loss of viability was associated with symptoms of a ripening disorder known as berry shrivel. FDA fluorescence of berry cells was rapid, bright, and stable for over 1 h at room temperature. Confocal microscopy detected FDA staining through two to three intact surface cell layers (300-400 mum) of bisected berries, and showed that the fluorescence was confined to the cytoplasm, indicating the maintenance of integrity in both cytoplasmic as well as vacuolar membranes, and the presence of active cytoplasmic esterases. FDA clearly discriminated between living cells and freeze-killed cells, and exhibited little, if any, non-specific staining. Propidium iodide and DAPI, both widely used to assess cell viability, were unable to discriminate between living and freeze-killed cells, and did not specifically stain the nuclei of dead cells. For normally developing berries under field conditions there was no evidence of viability loss until about 40 d after veraison, and the majority (80%) of mesocarp cells remained viable past commercial harvest (26 degrees Brix). These results are inconsistent with current models of grape berry development which hypothesize that veraison is associated with a general loss of compartmentation in mesocarp cells. The observed viability loss was primarily in the locule area around the seeds, suggesting that a localized loss of viability and compartmentation may occur as part of normal fruit development. The cell viability of berry shrivel-affected berries was similar to that of normally developing berries until the onset of visible symptoms (i.e. shrivelling), at which time viability declined in visibly shrivelled berries. Berries with extensive shrivelling exhibited very low cell viability (15%).

摘要

用二乙酸荧光素(FDA)作为一种活体染色剂,来检测发育中的葡萄(欧亚种葡萄)浆果中果皮组织的膜完整性(细胞活力),以验证以下假设:在成熟过程中,这些细胞中的区室化会大量丧失。该技术还用于确定活力丧失是否与一种称为浆果皱缩的成熟障碍症状相关。浆果细胞的FDA荧光在室温下快速、明亮且稳定超过1小时。共聚焦显微镜在对半切开的浆果的两到三层完整表面细胞层(300 - 400微米)中检测到FDA染色,并表明荧光局限于细胞质,这表明细胞质膜和液泡膜的完整性得以维持,且存在活性细胞质酯酶。FDA能清晰地区分活细胞和冻杀细胞,并且几乎没有非特异性染色。广泛用于评估细胞活力的碘化丙啶和DAPI无法区分活细胞和冻杀细胞,也不能特异性地对死细胞的细胞核进行染色。对于田间条件下正常发育的浆果,直到转色后约40天才有活力丧失的迹象,并且大多数(80%)中果皮细胞在商业采收(26°波美度)后仍保持活力。这些结果与当前的葡萄浆果发育模型不一致,当前模型假设转色与中果皮细胞中区室化的普遍丧失有关。观察到的活力丧失主要发生在种子周围的子房区域,这表明活力和区室化的局部丧失可能是正常果实发育的一部分。受浆果皱缩影响的浆果的细胞活力与正常发育的浆果相似,直到出现明显症状(即皱缩)时,此时明显皱缩的浆果中的活力下降。有广泛皱缩的浆果表现出非常低的细胞活力(15%)。

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