拟南芥砷酸还原酶基因AtACR2的表达调控及其功能分析

将砷酸盐还原为亚砷酸盐是植物砷代谢途径中的关键步骤，其中砷酸还原酶是催化砷酸盐还原的关键酶。目前，对植物中砷酸还原酶基因的表达调控机制及该基因的功能了解得还不是很清楚。因此研究拟南芥砷酸还原酶基因的表达调控及其功能对于探讨植物对砷吸收、代谢、转运和富集的分子机制有重要意义。 本论文利用拟南芥砷酸还原酶基因（AtACR2）的启动表达调控序列的不同组合驱动GUS基因转录表达，对AtACR2启动表达调控序列的功能进行了分析；同时利用过表达、AtACR2基因T-DNA插入缺失突变体和地上部特异表达对拟南芥和蜈蚣草砷酸还原酶的基因功能进行了初步分析，主要结果如下： 1．对拟南芥AtACR2基因在不同砷酸盐处理浓度(0、100 yM、200 yM) 下的RT-PCR分析初步表明：在未用Na3As04处理的拟南芥幼苗中，AtACR2基因在根和茎叶中均有表达，且其在根中的转录水平高于茎叶中。同时该基因的表达在转录水平上受砷酸盐的负调控，即随着外界砷酸盐浓度的升高，AtACR2基因的转录水平降低。 2．将AtACR2基因不同启动调控序列组合驱动GUS基因转录表达，结果表 明：①由AtACR2基因上游1250 bp及其5’端非编码医构成的启动调控序列不足以启动AtACR2基因的转录表达和砷酸盐胁迫的应答；②在第一外显子和第一内含子中存在启动AtACR2基因起始转录表达的关键序列元件，它们的存在决定了该基因能否得以转录表达；⑧第一外显子和第一内含子序列中不仅存在起始基因转录的必需元件，还存在砷胁迫相关的应答元件，参与砷酸盐抑制AtACR2基因的转录表达调控；④在第二外显子和第二内含子中可能存在增强基因表达的调控元件序列，进一步影响该基因转录表达强度的调控。 3． 拟南芥AtA CR2基因和砷超富集植物蜈蚣草PvA CR2基因在拟南芥中过表达后的功能分析初步表明：①转基因植株能够通过减少体内As含量增强对砷酸盐的抗性；②两种植物的砷酸还原酶作用能力存在一定差异，其中超表达蜈蚣草PvA CR2能够使转基因植株根中As含量更少，但其对砷酸盐胁迫的抗性并没有AtACR2超表达植株强，这可能与转 PvA CR2基因植株地上部积累相对较高的砷含量有关。 4．将AtA CR2和PvA CR2在拟南芥中地上部特异表达后，抗性实验初步表明：①以野生型拟南芥为背景材料进行地上部特异超表达AtACR2或PvA CR2基因，不能增强转基因植株对砷酸盐抗性；②以AtA CR2基因的T-DNA插入缺失突变体为背景材料地上部特异表达AtACR2或PvA CR2基因，却能够明显增强转基因植株对砷酸盐的抗性。综上所述，植物砷酸还原酶基因在植物对砷酸盐胁迫的响应和调控中起着重要作用。

Effects of arsenate on the growth and microcystin production of Microcystis aeruginosa isolated from Taiwan as influenced by extracellular phosphate

Arsenic pollution and eutrophication are both prominent issues in the aquaculture ponds of Taiwan. It is important to study the effects of arsenic on algal growth and toxin production in order to assess the ecological risk of arsenic pollution, or at least to understand naturally occurring ponds. The sensitivity of algae to arsenate has often been linked to the structural similarities between arsenate and phosphate. Thus, in this study we examined the effects of arsenate (10(-8) to 10(-4) M) on Microcystis aeruginosa TY-1 isolated from Taiwan, under two phosphate regimes. The present study showed that M. aeruginosa TY-1 was arsenate tolerant up to 10(-4) M, and that this tolerance was not affected by extracellular phosphate. However, it seems that extracellular phosphate contributed to microcystin production and leakage by M. aeruginosa in response to arsenate. Under normal phosphate conditions, total toxin yields after arsenate treatment followed a typical inverted U-shape hormesis, with a peak value of 2.25 +/- 0.06 mg L-1 in the presence of 10(-7) M arsenate, whereas 10(-8) to 10(-6) M arsenate increased leakage of similar to 75% microcystin. Under phosphate starvation, total toxin yields were not affected by arsenate, while 10(-6) and 10(-5) M arsenate stimulated microcystin leakage. It is suggested that arsenate may play a role in the process of microcystin biosynthesis and excretion. Given the arsenic concentrations in aquaculture ponds in Taiwan, arsenate favors survival of toxic M. aeruginosa in such ponds, and arsenate-stimulated microcystin production and leakage may have an impact on the food chain.

Effects of Arsenate on Microcystin Content and Leakage of Microcystis Strain PCC7806 Under Various Phosphate Regimes

Both arsenic pollution and eutrophication are prominent environmental issues when considering the problem of global water pollution. It is important to reveal the effects of arsenic species on cyanobacterial growth and toxin yields to assess ecological risk of arsenic pollution or at least understand naturally occurring blooms. The sensitivity of cyanobacteria to arsenate has often been linked to the structural similarities of arsenate and phosphate. Thus, we approached the effect of arsenate with concentrations from 10(-8) to 10(-4) M on Microcystis strain PCC7806 under various phosphate regimes. The present study showed that Microcystis strain PCC7806 was arsenate tolerant up to 10(-4) M. And such tolerance was without reference to both content of intra- and extra-cellular phosphate. It seems that arsenate involved the regulation of microcystin synthesis and cellular polyphosphate contributed to microcystin production of Microcystis responding to arsenate, since there was a positive linear correlation of the cellular microcystin quota with the exposure concentration of arsenate when the cells were not preconditioned to phosphate starvation. It is presumed that arsenate could help to actively export microcystins from living Microcystis cells when preconditioned to phosphate starvation and incubated with the medium containing 1 mu M phosphate. This study firstly provided evidence that microcystin content and/or release of Microcystis might be impacted by arsenate if it exists in harmful algal blooms. (C) 2008 Wiley Periodicals, Inc. Environ Toxicol 24:97 94, 2009.

Impacts of elevated CO2 concentration on biochemical composition, carbonic anhydrase, and nitrate reductase activity of freshwater green algae

To investigate the biochemical response of freshwater green algae to elevated CO2 concentrations, Chlorella pyrenoidosa Chick and Chlamydomonas reinhardtii Dang cells were cultured at different CO2 concentrations within the range 3-186 μ mol/L and the biochemical composition, carbonic anhydrase (CA), and nitrate reductase activities of the cells were investigated. Chlorophylls (Chl), carotenoids, carbonhydrate, and protein contents were enhanced to varying extents with increasing CO2 concentration from 3-186 μ mol/L. The CO2 enrichment significantly increased the Chl a/Chl b ratio in Chlorella pyrenoidosa, but not in Chlamydomonas reinhardtii. The CO2 concentration had significant effects on CA and nitrate reductase activity. Elevating CO2 concentration to 186 μ mol/L caused a decline in intracellular and extracellullar CA activity. Nitrate reductase activity, under either light or dark conditions, in C. reinhardtii and C. pyrenoidosa was also significantly decreased with CO2 enrichment. From this study, it can be concluded that CO2 enrichment can affect biochemical composition, CA, and nitrate reductase activity, and that the biochemical response was species dependent.