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生理和蛋白质组学分析揭示重金属 Cd 和 Zn 对烟草叶片中叶绿素、类胡萝卜素代谢和光合作用功能的毒性影响。

Toxic effects of heavy metal Cd and Zn on chlorophyll, carotenoid metabolism and photosynthetic function in tobacco leaves revealed by physiological and proteomics analysis.

机构信息

College of Resources and Environment, Northeast Agricultural University, Harbin, Heilongjiang, China; Key Laboratory of Saline-alkali Vegetation Ecology Restoration, Ministry of Education, College of Life Sciences, Northeast Forestry University, Harbin, Heilongjiang, China.

College of Resources and Environment, Northeast Agricultural University, Harbin, Heilongjiang, China.

出版信息

Ecotoxicol Environ Saf. 2020 Oct 1;202:110856. doi: 10.1016/j.ecoenv.2020.110856. Epub 2020 Jul 3.

Abstract

To explore the mechanisms underlying the action of the heavy metals Cd and Zn on the photosynthetic function of plant leaves, the effects of 100 μmol L Cd and 200 μmol L Zn stress (the exposure concentrations of Cd and Zn in the culture medium were 2.24 mg kg and 5.36 mg kg) on the chlorophyll and carotenoid contents as well as the photosynthetic function of tobacco leaves (Long Jiang 911) were studied. The key proteins in these physiological processes were quantitatively analyzed using a TMT-based proteomics approach. Cd stress was found to inhibit the expression of key enzymes during chlorophyll synthesis in leaves, resulting in a decrease of the Chl content. However, Zn stress did not significantly influence the chlorophyll content. Leaves adapted to Zn stress by upregulating CAO expression and increase the Chl b content. Although the Car content in leaves did not significantly change under either Cd or Zn stress, the expressions of ZE and VDE during Car metabolism decreased significantly under Cd stress. This was accompanied by damages to the xanthophyll cycle and the NPQ-dependent energy dissipation mechanism. In contrast, under Zn stress, leaves adapted to Zn stress by increasing the expression of VDE, thus improving NPQ. Under Cd stress, the expressions of three sets of proteins were significantly down-regulated, including PSII donor-side proteins (PPD3, PPD6, OEE1, OEE2-1, OEE2-2, OEE2-3, and OEE3-2), receptor-side proteins (D1, D2, CP43, CP47, Cyt b559α, Cyt b559β, PsbL, PsbQ, PsbR, Psb27-H1, and Psb28), and core proteins of the PSI reaction center (psaA, psaB, psaC, psaD, psaE-A, PsaE-B, psaF, psaG, psaH-1, psaK, psaL, psaN, and psaOL). In comparison, only eight of the above proteins (PPD6, OEE3-2, PsbL, PsbQ, Psb27-H1, psaL, and psaOL) were significantly down-regulated by Zn stress. Under Cd stress, both the donor side and the receptor side of PSII were damaged, and PSII and PSI experienced severe photoinhibition. However, Zn stress did not decrease either PSII or PSI activities in tobacco leaves. In addition, the expression of electron transport-related proteins (cytb6/f complex, PC, Fd, and FNR), ATPase subunits, Rubisco subunits, and RCA decreased significantly in leaves under Cd stress. However, no significant changes were observed in any of these proteins under Zn stress. Although Cd stress was found to up-regulate the expressions of PGRL1A and PGRL1B and induce an increase of PGR5/PGRL1-CEF in tobacco leaves, NDH-CEF was significantly inhibited. Under Zn stress, the expressions of ndhH and PGRL1A in leaves were significantly up-regulated, but there were no significant changes in either NDH-CEF or PGR5/PGRL-CEF. Under Cd stress, the expressions of proteins related to Fd-dependent nitrogen metabolism and reactive oxygen species (ROS) scavenging processes (e.g., FTR, Fd-NiR, and Fd-GOGAT) were significantly down-regulated in leaves. However, no significant changes of any of the above proteins were identified under Zn stress. In summary, Cd stress could inhibit the synthesis of chlorophyll in tobacco leaves, significantly down-regulate the expressions of photosynthesis-related proteins or subunits, and suppress both the xanthophyll cycle and NDH-CEF process. The expressions of proteins related to the Fd-dependent nitrogen metabolism and ROS scavenging were also significantly down-regulated, which blocked the photosynthetic electron transport, thus resulting in severe photoinhibition of both PSII and PSI. However, Zn stress had little effect on the photosynthetic function of tobacco leaves.

摘要

为了探索重金属 Cd 和 Zn 对植物叶片光合作用功能的作用机制,研究了 100 μmol·L Cd 和 200 μmol·L Zn 胁迫(培养基中 Cd 和 Zn 的暴露浓度分别为 2.24 mg·kg 和 5.36 mg·kg)对烟草(龙烟 911)叶片叶绿素和类胡萝卜素含量以及光合作用功能的影响。使用 TMT 基于蛋白质组学方法定量分析了这些生理过程中的关键蛋白质。结果表明,Cd 胁迫抑制了叶片中叶绿素合成过程中的关键酶的表达,导致 Chl 含量降低。然而,Zn 胁迫对 Chl 含量没有显著影响。叶片通过上调 CAO 表达和增加 Chl b 含量来适应 Zn 胁迫。虽然 Cd 或 Zn 胁迫下叶片中的 Car 含量没有显著变化,但 Car 代谢过程中 ZE 和 VDE 的表达显著下降。这伴随着叶黄素循环和 NPQ 依赖的能量耗散机制的破坏。相比之下,在 Zn 胁迫下,叶片通过增加 VDE 的表达来适应 Zn 胁迫,从而提高 NPQ。在 Cd 胁迫下,三组蛋白质的表达显著下调,包括 PSII 供体侧蛋白(PPD3、PPD6、OEE1、OEE2-1、OEE2-2、OEE2-3 和 OEE3-2)、受体侧蛋白(D1、D2、CP43、CP47、Cyt b559α、Cyt b559β、PsbL、PsbQ、PsbR、Psb27-H1 和 Psb28)和 PSI 反应中心的核心蛋白(psaA、psaB、psaC、psaD、psaE-A、PsaE-B、psaF、psaG、psaH-1、psaK、psaL、psaN 和 psaOL)。相比之下,只有上述八种蛋白质(PPD6、OEE3-2、PsbL、PsbQ、Psb27-H1、psaL 和 psaOL)在 Zn 胁迫下显著下调。在 Cd 胁迫下,PSII 的供体侧和受体侧均受到损伤,PSII 和 PSI 经历了严重的光抑制。然而,Zn 胁迫并没有降低烟草叶片中的 PSII 或 PSI 活性。此外,在 Cd 胁迫下,电子传递相关蛋白(cytb6/f 复合物、PC、Fd 和 FNR)、ATP 酶亚基、Rubisco 亚基和 RCA 的表达显著下降。然而,在 Zn 胁迫下,这些蛋白质中没有任何一种的表达发生显著变化。虽然 Cd 胁迫被发现可以上调 PGRL1A 和 PGRL1B 的表达,并诱导烟草叶片中 PGR5/PGRL1-CEF 的增加,但 NDH-CEF 受到显著抑制。在 Zn 胁迫下,叶片中 ndhH 和 PGRL1A 的表达显著上调,但 NDH-CEF 或 PGR5/PGRL-CEF 没有显著变化。在 Cd 胁迫下,与 Fd 依赖的氮代谢和活性氧(ROS)清除过程相关的蛋白质(如 FTR、Fd-NiR 和 Fd-GOGAT)的表达显著下调。然而,在 Zn 胁迫下,没有观察到上述任何一种蛋白质的表达发生显著变化。综上所述,Cd 胁迫可以抑制烟草叶片中叶绿素的合成,显著下调光合作用相关蛋白或亚基的表达,并抑制叶黄素循环和 NDH-CEF 过程。与 Fd 依赖的氮代谢和 ROS 清除相关的蛋白质的表达也显著下调,这阻断了光合作用电子传递,从而导致 PSII 和 PSI 严重的光抑制。然而,Zn 胁迫对烟草叶片的光合作用功能几乎没有影响。

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