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Interactive effects of selenium and arsenic on growth, antioxidant system, arsenic and selenium species of Nicotiana tabacum L.
Accepted Manuscript Title: Interactive effects of selenium and arsenic on growth, antioxidant system, arsenic and selenium species of Nicotiana tabacum L. Author: Dan Han Shuanglian Xiong Shuxin Tu Jinchang Liu Cheng Chen PII: DOI: Reference:
S0098-8472(15)00081-7 http://dx.doi.org/doi:10.1016/j.envexpbot.2015.04.008 EEB 2927
To appear in:
Environmental and Experimental Botany
Received date: Revised date: Accepted date:
15-11-2014 4-4-2015 14-4-2015
Please cite this article as: Han, Dan, Xiong, Shuanglian, Tu, Shuxin, Liu, Jinchang, Chen, Cheng, Interactive effects of selenium and arsenic on growth, antioxidant system, arsenic and selenium species of Nicotiana tabacum L.Environmental and Experimental Botany http://dx.doi.org/10.1016/j.envexpbot.2015.04.008 This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Interactive effects of selenium and arsenic on growth, antioxidant system, arsenic and
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selenium species of Nicotiana tabacum L.
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First name: Dan; Family name: Hana, b, c
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First name: Shuanglian; Family name: Xionga, b, c
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First name: Shuxin; Family name: Tua, b, c
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First name: Jinchang; Family name: Liua, b, c
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First name: Cheng; Family name: Chena, b, c
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a
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430070, China
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b
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China
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c
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Yangtze River), Ministry of Agriculture, Wuhan 430070, China
College of Resources and Environment, Huazhong Agricultural University, Wuhan
Microelement Research Center, Huazhong Agricultural University, Wuhan 430070,
Key Laboratory of Arable Land Conservation (Middle and Lower Reaches of
16 17
Corresponding author
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Shuanglian Xiong; College of Resources and Environment, Huazhong Agricultural
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University, Wuhan 430070, China; Tel.: +86 027 87282137 fax: +86 027 87288618.
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E-mail: [email protected] (S. Xiong).
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Shuxin Tu; College of Resources and Environment, Huazhong Agricultural University,
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Wuhan 430070, China. E-mail: [email protected] (S. Tu).
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Highlights
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●
The moderate dose of Se/As in solution promoted the growth of FCT.
25
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Different Se/As levels in solution affects the ratios of Se/As species of FCT.
26
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Se mitigates As toxicity by improving the antioxidant capacity.
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Se mitigates As toxicity by influencing on the Se/As species of FCT changes.
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Abstract
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This paper is aimed to study separate and interactive effects of selenium (Se) (selenite,
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0-5 mg L-1) and arsenic (As) (arsenate, 0-5 mg L-1) on the growth and the antioxidant
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system of flue-cured tobacco (FCT) as well as the contents and species of As and Se
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in FCT through a hydroponic experiment and clarify the possible mechanism how Se
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alleviates the toxicity of As. The results were: single addition of Se (≤ 1 mg L-1) or As
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(1 mg L-1) by a low dose could stimulate the growth of FCT, but the growth of FCT
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would be inhibited when Se (5mg L-1) or As (5mg L-1) was added by a high dose. Low
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As levels stimulated the uptake of Se but high levels of As posing the opposite effects
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with the low Se dosage. However, the addition of As always inhibited the uptake of Se
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with high Se levels. Moreover, Se showed dual effects on the uptake of As. At the low
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As dose (1mg L-1), the addition of Se inhibited the growth of FCT, but significantly
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promoted the activity of superoxide dismutase (SOD) and peroxidase (POD) enzymes
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as well as the content of MDA. Meanwhile, the percentages of organic Se and As(III)
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in the leaves of FCT declined with the increasing Se dose. However, the addition of
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Se by a moderate dose (0.1mg L-1) alleviated the toxicity of the high As dose (5mg L-1 )
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and promoted the growth of FCT by elevating the ability of anti-oxidative stress of
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FCT and reducing the contents of MDA and As in FCT. The Se species in the leaves
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of FCT existed in organic ones (SeCys and SeMet) (100%), while the major As
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speciation was As(III) (75%). Likewise, the addition of As counteracted the toxicity of
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high Se dose (5 mg L-1) and promoted the growth of FCT slightly as it reduced the
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formation of organic Se or failed to transform excess inorganic Se species into organic
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ones and depressed the contents of Se in the roots and leaves of FCT. In a word, the
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low Se dose (0.1mg L-1) alleviated of the toxicity of the high As dose and the addition 2
53
of As counteracted the toxicity of high Se dose (5 mg L-1), as a result of which the
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promotion of the growth of FCT were realized.
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Keywords: Arsenate; Selenite; Interaction; Antioxidant system; Species.
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Abbreviations: Se, selenium; As, arsenic; MDA, malondialdehyde; SOD, superoxide dismutase;
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POD, peroxidase; AsA, ascorbate acid; GSH, glutathione; As(V),arsenate; As(III), arsenite; ROS,
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reactive oxygen species; MMA, monomethylarsonicacid; DMA, dimethylarsinic acid; Cd,
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cadmium; Hg, mercury; Ni, nickel; Pb, lead; GR, glutathione reductase; Se(IV), selenite; Se(VI),
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selenate; SeCys, selenocysteine; SeMet, selenomethionine; AR, arsenate reductase; PC,
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phytochelatins.
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1. Introduction
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Arsenic (As) is a severe pollutant which is highly toxic to animals and plants and
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widely distributes in the environment. Arsenic exists in the forms of arsenate [As(V)],
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arsenite [As(III)], monomethylarsonic acid [MMA] and dimethylarsinic acid [DMA],
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but As(V) and As(III) are the main species (Tripathi et al., 2007; Zheng et al., 2013),
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which mainly come from mining, coal ash, dust, off gas, pesticides and sewage
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sluge(Meunier et al., 2011; Saunders et al., 2010). The accumulation of As in soil
70
doesn’t only can affect the growth and development of plants, but also pose a threat to
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human health via the food chain. Arsenic impedes the photosynthesis and reduces the
72
contents of essential nutrients, thus inhibits the growth of crops and even causes them
73
death (Garg and Singla, 2011). For human, arsenic may lead to cancerous and
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non-cancerous diseases, including bladder cancer, lung cancer, liver cancer and so on
75
(Farnese et al., 2014).
76
Although there is no evidence that selenium (Se) is an essential element for plants so
77
far, it is an essential microelement for human and animals. An appropriate dose of Se
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can improve the antioxidant capacity, scavenge excessive oxygen free radicals,
79
decrease lipid peroxidation, defer senescence, promoting the growth of plants (Lin et
80
al., 2012), and detoxify heavy metals (metalloids) in plants, for example arsenic (As)
81
(Malik et al., 2012), cadmium (Cd)(Feng et al., 2012; Lin et al., 2012; Saidi et al.,
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2014), mercury (Hg) (Zhang et al., 2012a), nickel (Ni) (Gajewska et al., 2013) and
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lead (Pb) (Mroczek-Zdyrska and Wojcik, 2012). Currently, the researches on the
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mechanism how Se mitigates the toxicity of As are mainly concentrated on the
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elimination of reactive oxygen species (ROS), the suppression of lipid peroxidation
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and the enhancement of the antioxidant capacity of plants(Kramárová et al., 2012;
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Malik et al., 2012). Se exists mainly in the forms of Se(IV), selenate Se (VI),
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selenocysteine (SeCys) and selenomethionine (SeMet) in plants (Zhu et al., 2009).
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After absorbed by plants, Se(IV) or Se(VI) is converted into other forms like
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selenocysteine (SeCys) and selenomethionine (SeMet) (Zhu et al., 2009). Moreover, 4
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Se can replace sulphur in the amino acids as SeMet and SeCys due to their
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physicochemical similarity. And the organic Se species (SeCys and SeMet) can be
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incorporated into proteins, replacing cysteine (Cys) and methionine (Met),
94
respectively, which can result in toxicity in plants (Navarro-Alarcon and
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Cabrera-Vique, 2008; White et al., 2004). However, the toxicity of soluble inorganic
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As is greater than that of organic As, and the toxicity of As(III) is higher than that of
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As(V) in the environment (Yamauchi, 1994; Yin et al., 2013). Having taken up by the
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roots of plants via the phosphate transport pathway (Wu et al., 2011b; Zhao et al.,
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2010), As(V) can be rapidly reduced to As (III) by arsenate reductase (AR) (Zhao et
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al., 2009). As(III), which can also be taken up by the roots of plants mainly through
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silicic acid transport protein (Ma et al., 2008), is chelated with polypeptides like GSH
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and PCs and finally stored in the vacuoles of roots to detoxify As(Liu et al., 2010; Ye
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et al., 2011; Zhang et al., 2012c). A previous study showed that Se could mitigate the
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toxicity of As via antagonistic effects in Pteris vittata (Feng et al., 2009).
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However, the changes of As and Se species in plants under the exposure of As and Se
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are still unclear. We infer that Se can mitigate the toxicity of As by regulating the
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antioxidant system and simultaneously affecting As species in plants.
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Tobacco leaf, which contains abundant and high-quality soluble proteins (Teng and
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Wang, 2012), is considered as an ideal material to produce Se-rich protein. In this
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study, Nicotiana tabacum L. was chosen as the test material to investigate: (1) the
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responses of the growth and antioxidant systems of FCT to different doses of Se and
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As; (2) the relation among the variations of As species and the detoxification of As
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after Se supplementation.
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2. Materials and methods
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2.1. Seedling cultivation
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The cultivar was N. tabacum K326, and the floating cultivation method was adopted
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for the cultivation of seedlings. Later, the seedlings of similar sizes were transplanted 5
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into plastic pots containing 10 L nutrient solution which was composed of 4 mmolL-1
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Ca(NO3)2·4H2O, 5 mmolL-1 KNO3, 1mmolL-1 NH4H2PO4, 2 mmolL-1 MgSO4·7H2O,
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0.01 mmolL-1 EDTA-Fe, 0.046 mmolL-1 H3BO3, 0.0008 mmolL-1 ZnSO4·7H2O and
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0.0003 mmolL-1 CuSO4·5H2O. The plants grew in a greenhouse with natural light at
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25-30℃.
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2.2. Experimental design and implementation
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A hydroponic experiment of four Se levels, i.e. 0, 0.1, 1.0 and 5.0 mg L-1, and three
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As levels, i.e. 0, 1.0 and 5.0 mg L-1, was designed. As and Se were added in the forms
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of Na3AsO4.12H2O and Na2SeO3, respectively. A randomized complete block design
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was employed. There was a total of 12 treatments, namely CK (without the addition
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of Se and As), Se0.1As0, Se1As0, Se5As0, Se0As1, Se0.1As1, Se1As1, Se5As1,
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Se0As5, Se0.1As5, Se1As5 and Se5As5, and each treatment was repeated for three
130
times.
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Four-leaf FCT seedlings were transplanted to 1/4 strength Hoagland-Arnon nutrient
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solution at first and three days later, the solution was replaced by 1/2 strength nutrient
133
and the nutrient solution was renewed every five days. After forty days, the seedlings
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of even size were transplanted to the plastic cases (22×16×7cm) and subject to the
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above-mentioned Se and/or As treatments with full strength Arnon-Hoagland nutrient
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solution, and each pot contained 2 plants. The plants were harvested after fourteen
137
days. After rinsed carefully with tap water and deionized water successively, the
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separated fresh leaves and roots were weighed and divided into two parts. One was
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immersed in N2 liquid immediately and stored at -80℃ to determine the Se and As
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species and the indices of the antioxidant systems later. The other was over-dried at
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105°C for 15 min to de-enzyme at first, and then at 65°C for 48 h and finally
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pulverized to determine the contents of As and Se.
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2.3. Determination of Se and As contents and species
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The contents of Se and As were determined with a hydride generation atomic
145
fluorescence spectrometer (AFS8220, Beijing Titan Instruments Co., China) (Feng et
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al., 2009a) after the tissues of FCT were digested with concentrated HNO3-HClO4.
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The accuracy of elemental analysis was verified by standard reference materials
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[GBWO7602 (GSV-1)] from the Center for Standard Reference of China.
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A methanol: water (1:2) method was used to extract Se species in leaves or roots of
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FCT plants. The separation of SeIV, SeVI, SeMet and SeCys in the green parts of FCT
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was carried out with a anion exchange chromatography in which the column was
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connected to a ultraviolet treatment-hydride generation atomic fluorescence
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spectrometry (UV-HG-AFS) detection system (Han et al., 2013) online.
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The extraction of As species was similar to that of Se species. Because no organic
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arsenic in FCT were detected in a preliminary experiment, only As(V) and As(III)
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were measured in this study. The separation of As(V) and As(III) in leaves and roots
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of FCT plants was conducted with the anion exchange chromatography in which the
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column was also connected to the HG-AFS detection system (Zhang et al., 2002)
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online.
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The HPLC system consisted of a SHIMADZU 10ATvp Plus liquid chromatography
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pump (SHIMADZU, Tokyo, Japan), a Rheodyne 7725i injector (Rheodyne, Cotati,
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USA) and a Hamilton PRP-X100 column (Hamilton, Reno, NV). The mobile phase
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for HPLC was 15 mmol L-1(NH4)2HPO4 (pH 6.0, 1.0 mL min-1). As for the HG phase,
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the reduction agents were 1.5% KBH4 (m/v)+0.5% KOH (m/v) and the carrier
165
solution was 7% HCl (v/v). The detection phase was AFS8220, with the Se hollow
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cathode lamp current (General Research Institute for Nonferrous Metals, Beijing,
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China) of 50 mA, the negative high voltage of photomultiplier tube of 270V, the flow
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rate of carrier gas of 400 mL min-1 and the flow rate of makeup gas of 600 mL min-1.
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2.4. Assay of enzymatic and non-enzymatic antioxidants
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The activity of superoxide dismutase (SOD) was determined with the method put
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forward by Zhang et al.(Zhang et al., 2012b). In brief, 0.5g fresh FCT leaves was
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grounded in 5mL extraction buffer containing 50 mM potassium phosphate (pH7.8) at
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first, and then the homogenate was centrifuged at 10,000×g for 15 min at 4°C. 3mL
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reaction mixture contained 13 mM methionine, 75 μM NBT, 2 μM riboflavin, 0.1 mM
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EDTA and 100μL enzyme extract. The reaction mixture was illuminated for 15 min.
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The sample absorbance was determined at 560 nm, and the unit SOD activity was
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defined as the amount of enzyme to inhibit 50% of the NBT reduction.
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The activity of peroxidase (POD) was measured with the method described by Zhang
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et al. (Zhang et al., 2012b). In brief, 0.5g fresh leaves of FCT were extracted with 5
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mL 50mM potassium phosphate buffer (pH 5.5). Afterwards, the extracts were
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centrifuged at 10,000×g for 15min at 4°C. The reaction mixture contained 1 mL
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extraction buffer, 5μL 30% H2O2, 5μL guaiacol and 15μL supernatant. The molar
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extinction coefficient of 26.6 mM−1cm−1 was used for the calculation of the enzyme
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activity.
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Ascorbate (AsA) was extracted from 0.5g FCT leaves with 10g L−1 oxalic acid and
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determined spectrophotometrically with 2,4-dinitrophenylhydrazine colorimetry
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method proposed by Zhang et al. (Zhang et al., 2012b). 0.5g samples were
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homogenized with 3% metaphosphoric acid at first, then the homogenate was
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centrifuged for 10min at 10,000×g and finally the supernatant was used for
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glutathione (GSH) assays (Zhang et al., 2012b).
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The MDA content was assayed with 2.5 mL solution of 20% (w/v) trichloroacetic acid,
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which included 0.5% (w/v) thiobarbituric acid and 1.5 mL enzyme extract. The
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solution was kept in boiling water for 20min bath at first and then cooled quickly.
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After refrigeration, the homogenate was centrifuged at 5,000 g for 10 min at 25°C.
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The absorbances of supernatant were recorded at 532 nm and 600 nm, respectively.
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The absorbance at 600 nm was subtracted from that at 532 nm. The MDA content was
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calculated based on the extinction coefficient of MDA, namely 155 mM−1cm−1(Feng 8
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et al., 2009b).
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2.5. Statistical analysis
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All data were subject to two-way ANOVA analysis and Tukey's multi-comparisons
201
test (P≤0.05). The results were expressed as the means and the corresponding standard
202
errors. All statistical analyses were completed using the SAS 8.1 software.
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3. Results
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3.1. Growth of FCT
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Without the addition of As, low Se levels (≤ 1mg L-1Se) stimulated the growth of FCT,
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but high Se levels (5 mg L-1) had the opposite effects on and inhibited the growth of
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FCT compared with the CK treatment (Fig. 1AB). The fresh weights of leaves and
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roots of FCT in Se5As0 treatment were 32% and 43% of those of the CK treatment,
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respectively (Fig. 1AB). Similarly, in the absence of Se, 1mg L-1 As stimulated the
210
growth of FCT, but 5mg L-1As significantly hindered the growth of FCT, especially
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the roots of FCT (Fig. 1AB). The fresh weights of leaves and roots of FCT in Se0As1
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treatment were 22% and 24% higher than those in the CK treatment, respectively. The
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fresh weight of roots in Se0As5 treatment was 24% lower than that in the CK
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treatment (Fig. 1AB).
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Under low As treatments (1 mg L-1 As), the addition of Se inhibited the growth of FCT
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(Fig. 1AB). The fresh weights in Se0.1As1, Se1As1 and Se5As1 treatments were 91%,
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68%, 38% (for leaves) and 88%, 108%, 35% (for roots) of those in Se0As1 treatment,
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respectively. However, at the high As level (5mg L-1), the low Se level (0.1mg L-1Se)
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enhanced but high Se level (5mg L-1Se) obviously depressed the growth of FCT (Fig.
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1AB). For example, the fresh weights of shoots and roots in Se0.1As5 treatment were
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1.1 times and 1.5 times of those in Se0As5 treatment, respectively. Nevertheless, the
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fresh weights of shoots and roots in Se5As5 treatment were 40% and 75% of those in
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Se0As5 treatment, respectively (Fig. 1AB).
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3.2. Uptake, distribution and species of Se or As of FCT
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At a certain As dose, the contents of Se in the leaves and roots of FCT went up along
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with the increasing Se level (Fig. 2AB).
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Se and As had significant interactive effects on the contents of Se in leaves and roots
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of FCT (F=79.26 and 81.06, P<0.01, respectively). The effects of As on the uptake of
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Se depended on the levels of Se and As in solution. At the low Se level (≤ 1 mg L-1), 1
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mg L-1 As promoted the uptake of Se by the leaves and roots of FCT, but 5 mg L-1As
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had negative effects on the uptake of Se.
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At the high Se level (5 mg L-1), As showed antagonistic effects on the uptake of Se in
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the leaves and roots of FCT. The contents of Se in the leaves and roots of FCT in
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Se5As1 and Se5As5 treatments were 82% and 69% (for roots), 66% and 61% (for
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leaves) of those in Se5As0 treatment, respectively (Fig. 2AB).
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At a certain Se level, the contents of As in the leaves and roots of FCT increased
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along with elevation of the As level significantly (Fig. 3AB), and in particular the
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content of As in roots was far higher than that in the leaves (Fig. 3AB).
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The interaction of Se and As had significant effects on the uptake of As by FCT
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(F=34.57 and 26.63, P<0.01, respectively). At 1 mg L-1 As level, the elevation of the
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Se levels raised the As content in the leaves (Fig. 3A) but failed to enhance the As
242
content in the roots of FCT. However, at 5 mg L-1 As level, the growth of Se level
243
remarkably reduced the contents of As in leaves and roots of FCT (Fig. 3AB).
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Only SeCys and Se(IV) were detected in the roots, whereas SeCys, SeMet and Se(IV)
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were observed in the leaves of FCT (Fig. 4AB). In 0.1 mg L-1 Se treatment, main Se
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species in the leaves of FCT were organic ones (SeCys and SeMet) (58%-100%),
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which gradually increased with the growth of the As level (Fig. 4A). Similarly, the
248
proportion of organic Se species (SeCys) in the roots of FCT went up from 30% to
249
69% with the growth of the As level (Fig. 4B).
250
In 1 mg L-1 Se treatment, the percentage of organic Se species declined in the leaves 10
251
but increased in the roots of FCT along with the elevation of the As level. To be
252
specific, the proportions of organic Se species (SeCys and SeMet) in the leaves
253
decreased from 68% (Se1As1) to 42% (Se1As5), while the percentage of organic Se
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species (SeCys) in the roots of FCT went up from 47% (Se1As1) to 84% (Se1As5).
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In 5 mg L-1 Se treatment, the percentages of organic Se species in the leaves and roots
256
of FCT decreased along with the elevation of the As level.
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In the leaves of FCT, As (V) was the main speciation at the low As level of 1mg L-1
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(63%-94%), whereas As(III) was the major As speciation at the high As level of 5mg
259
L-1 (63%-78%) (Fig.5A). At a certain As level, the proportion of As(III) in the leaves
260
of FCT declined along with the growth of the Se level. For example, the proportion of
261
As(III) in the leaves dropped from 37% to 6% at 1mg L-1 As but decreased from 74%
262
to 63% at 5mg L-1 As along with the elevation of the Se level.
263
As(III) was the main As speciation in the roots of FCT (Fig. 5B). At the low As level
264
(1mg L-1), 0.1mg L-1 Se reduced the proportion of As(III) in the roots of FCT but the
265
other Se levels raised the proportion of As(III) in comparison with the Se0As1
266
treatment. At the high As level (5mg L-1), the elevation of the Se level had no
267
significant effects on the proportions of As(III) and As (V) (Fig. 5B).
268
3.3. Antioxidant system of FCT under As/Se stress
269
Se and As treatments had great influences on the activities of SOD and POD (P<0.01).
270
Regardless of the addition of As, the addition of Se markedly increased the activities
271
of SOD and POD of the leaves of FCT (Fig. 6AB, P<0.05). However, whether Se is
272
added into the solution or not, the elevation of the As level significantly enhanced the
273
SOD activity but generally decreased the POD activity of the leaves of FCT except
274
that the POD activity was significantly enhanced at the Se level of 1 mg L-1 and along
275
with the growth of the As level (Fig. 6AB).
276
As and Se had significant influences on the GSH content in the leaves of FCT
277
(F=15.50, P<0.01). Without the addition of As in the solution, the growth of the Se
278
level significantly enhanced the GSH content in the leaves of FCT (Fig. 6C). 11
279
At a low As level of 1 mg L-1, the GSH content was also enhanced by increasing the
280
Se level except for the GSH content was reduced by 15% at the Se level of 1 mg L-1
281
compared with the Se0As1 treatment (Fig.6C). At the high As level of 5 mg L-1, the
282
GSH content did not significantly change with the increasing Se level (Fig. 6C).
283
When Se was not added in the solution, the increase of the As level significantly
284
enhanced the GSH content in the leaves of FCT. However, when Se was present in the
285
solution, the addition of As appeared to show insignificant effects on or reduce the
286
GSH content in FCT (Fig. 6C).
287
The interaction of Se and As significantly affected the AsA content in the leaves of
288
FCT (F=60.07, P<0.01). At a certain As level, the increasing Se levels significantly
289
raised the AsA content in the leaves of FCT. When no Se or 0.1 mg L-1 Se was added
290
in the solution, 1 mg L-1 As reduced but 5 mg L-1 As recovered or increased the AsA
291
content compared with the CK and Se0.1As0 treatments, respectively (Fig. 6D).
292
However, when 1 or 5 mg L-1 Se was added in the solution, 5 mg L-1 As significantly
293
enhanced the AsA content (Fig. 6D).
294
Se and As treatments could dramatically affect the MDA content (P<0.01). When no
295
As was added in the solution, 0.1 mg L-1 Se significantly reduced the MDA content in
296
the leaves of FCT but 1 and 5 mg L-1 Se enhanced the MDA content compared with
297
the CK treatment (Fig. 7). However, when Se was absent from the solution, 1 mg L-1
298
As reduced the MDA content in the leaves of FCT but 5 mg L-1 As resulted in the
299
reduction of the MDA content to the level in the CK treatment (Fig. 7).
300
When 1 mg L-1 As was added into the solution, the increasing Se level significantly
301
enhanced the MDA content in the leaves of FCT. However, with 5 mg L-1 As in the
302
solution, only 5 mg L-1 Se significantly enhanced the MDA content. In the presence of
303
0.1 mg L-1 Se in the solution, the addition of As did not significantly affect the MDA
304
content in FCT. However, when 1 or 5 mg L-1 Se was added in the solution, 1 mg L-1
305
As significantly enhanced but 5 mg L-1 significantly reduced the MDA content in the
306
leaves of FCT.
12
307
4. Discussion
308
This study attempted to illuminate the mechanism how Se detoxifies As via regulating
309
the antioxidant systems of FCT and the variations of species of As and Se in FCT. As
310
expected, the addition of Se can detoxify As, showing as the stimulated leaf and root
311
biomass of FCT exposed to high levels of As. However, this alleviation process might
312
be dependent on the dosages of Se and As, because the high Se level (5 mg L-1) had
313
already showed toxic effects on the plant growth whether As was added into the
314
solution or not. Furthermore, when plants were exposed to 1 mg L-1 As, the addition
315
of Se did not show beneficial but negative effects on the growth of FCT because the
316
addition of Se might counteract the beneficial effects of low As dosages on the growth
317
of FCT. Similar results have been reported by Malik et al. (2012) on mung bean
318
(Phaseolus aureus Roxb.) and Zhao et al. (2013b) on garlic (Allium sativum). With
319
increase in arsenic (As) concentration, a marked inhibition in the growth of plants was
320
observed. The plants treated 10 uM As (0.7 mg L-1) and supplemented with 2.5uM Se
321
(0.2 mg L-1) showed 22% growth improvement in shoots and 16% in roots compared
322
to those growing in As alone(Malik et al., 2012). Low-level exposure to Se(≤0.1 mg
323
L-1) or Hg (≤0.01 mg L-1) is beneficial for garlic growth, whereas Se(>1 mg L-1) or
324
Hg (>0.1 mg L-1) levels above certain threshold limits can be harmful. As for Se-Hg
325
co-exposed garlic, the stimulation of garlic growth by low levels of Se is also
326
enhanced by HgCl2 at low levels (≤0.1 mg L-1 Hg), by contrast, an antagonistic effect
327
between low levels of Se and higher Hg levels (1 mg L-1 or 10 mg L-1) is
328
observed(Zhao et al., 2013b).
329
Like the effects of As and Se of different levels on the growth of plant, the Se uptake
330
might also depend on the levels of As and Se in the solution. Low As levels stimulated
331
the uptake of Se but high levels of As appeared to bring about the opposite effects
332
when the plants were subject to low dosages of Se. However, when plants were
333
exposed to high Se levels, the addition of As always inhibited the uptake of Se.
334
Similar results about the uptake of As on Se have been reported on P. vittata (Feng et
13
335
al., 2009a) and garlic (Allium sativum) (Zhao et al., 2013a). The increased Se uptake
336
in FCT might be used to synthesize some important substances, such as GSH-Px
337
(glutathione peroxidase), and rebalance the excessive ROS, during which GSH will be
338
needed in huge doses, like the significant growth of the GSH content in this study (Fig.
339
6C). However, when As and Se was added in excess, some vital substances (for
340
example GSH) might not satisfy the metabolism demands of As and Se. Therefore,
341
there was a competition between As and Se to integrate with GSH, and they showed
342
the mutually antagonistic effects. The results above matched well with the hypothesis
343
of Feng et al. (2013). Interestingly, Se showed dual effects on the uptake of As in this
344
study. The exact reasons behind the stimulation of the As uptake in the leaves of FCT
345
subject to low As doses by Se were unknown (Fig. 3A). However, similar inhibition
346
effects of Se on the uptake of As were also reported on Phaseolus aureus Roxb.
347
(Malik et al., 2012) and Pteris vittata (Feng et al., 2009a). Se (SeO32- or SeO42-) at
348
high exposure levels (>1mg L-1) also significantly inhibited the uptake of Hg in
349
garlic when Hg2+ levels were higher than 1mg L-1 in the culture media (Zhao et al.,
350
2013a). Since As(V) and Se(IV) were taken up by roots via the phosphate transport
351
pathway(Wu et al., 2011a; Zhu et al., 2009), the antagonistic effects between Se and
352
As on their mutual uptakes might be related to their competition for binding sites.
353
The detoxification of As by Se might be also closely with the changes of As and Se
354
species. In the leaves of FCT, the addition of Se resulted in more accumulation of
355
As(V) and less accumulation of As(III) (Fig. 5A), but the opposite trends were
356
observed in the roots (Fig. 5B). It is well established that As(III) is more toxic than
357
As(V) in plants. Therefore, a conclusion could be drawn that Se could reduce the
358
toxicity of As since it reduced the transfer of As(III) from the roots to the
359
above-ground parts of plants.
360
When Se was added at low levels in the solution, organic Se species (SeCys and
361
SeMet) were predominant in the leaves of FCT, and the increasing As levels enhanced
362
the transformation of inorganic Se into organic Se (Fig. 4A), which might be related
363
with the antioxidative effects of low Se dosages (Feng et al., 2013). It was reported
364
that organic Se could directly quench ROS, especially hydroxylic free radical (OH•) 14
365
(Feng et al., 2013). Therefore, the enhancement of organic Se in the leaves of FCT
366
was conducive to the rebalance of ROS of plants. However, the proportion of
367
inorganic Se [Se(IV)] increased when FCT was subjected to the high levels of As and
368
Se. Se was considered as a pro-oxidant at high levels, and synthesized proteins in
369
place of S(Feng et al., 2013; Terry et al., 2000). Therefore, the more accumulation of
370
inorganic Se after the addition of high levels of Se and As might suggest that to avoid
371
the toxicity of high levels Se, plant will reduce the formation of organic Se or cannot
372
transform excess inorganic Se into organic over a short period of time. In addition, the
373
competition between As and Se to integrate with GSH might also a key influential
374
factor to the formation of organic Se, which was realized with the help of GSH (Feng
375
et al., 2013). Similar results have been reported by Han et al. (2013) on Nicotiana
376
tabacum L.. In the leaves and roots of FCT, the addition of Se resulted in more
377
accumulation of organic Se species at low Se levels and more accumulation of
378
inorganic Se species at high Se levels(Han et al., 2013). Moreover, Compared with
379
roots, shoots of all the three plants (alfalfa, maize, and soybean) had a higher
380
percentage of organic Se (especially SeCys) by using Se(IV)-spiked soil(Yu et al.,
381
2011).
382
As expected, Se could affect the antioxidant system and regulate the toxicity of As,
383
judged from the increased activities of SOD and POD and the enhanced contents of
384
GSH and AsA, suggesting that these antioxidants play important roles in the
385
detoxification of As by Se. However, Se also showed toxicity to FCT, as it increase
386
the MDA content (Fig.7), decreased the fresh weights of leaves and roots at high Se
387
levels (Fig.1AB). In line with the increased fresh weight of leaves (Fig.1A), the
388
decreased Se contents in the leaves and roots (Fig.2AB) and organic Se proportion
389
(Fig.4AB) as well as the enhanced SOD activity and contents of GSH and AsA, the
390
addition of As seemed to exert detoxification effects on the high Se level (5 mg L-1)
391
(Fig.4ACD).
15
392
5. Conclusion
393
The low Se level (0.1mg L-1Se) alleviated the toxicity of high As level (5 mg L-1) and
394
thus promoted the growth of FCT by regulating the antioxidant system and reducing
395
the transfer of As(III) from the roots to the above-ground parts of FCT. Likewise, the
396
addition of As counteracted the toxicity of high Se level (5 mg L-1) and promoted the
397
growth of FCT slightly because it reduced the formation of organic Se, failed to
398
transform excess inorganic Se into organic Se over a short period of time and
399
depressed the Se contents in roots and leaves of FCT.
400
Acknowledgments
401
This research was partially supported by National Science Foundation of China
402
(41101464) and National Special Fund for Agro-scientific Research in the Public
403
Interest (201303106).
404
405
406
407
408
409
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519 520 521 522 523 524 525 526 527 528 529 530 531 532 20
533
Fig.1. The biomass in shoots (A) and roots (B) of flue-cured tobacco treated with As
534
and Se for 14 days under hydroponic conditions. The values are mean ± SE (n = 3).
535
Different letters above bars indicate significant difference at P<0.05 (Capital letters
536
denote significance within the same arsenic level at different doses of selenium;
537
lowcase letters denote significance within the same selenium level at different doses
538
of arsenic).
539
Fig.2. The Se concentration in leaves (A) and roots (B) of flue-cured tobacco treated
540
with As and Se for 14 days under hydroponic conditions. The values are mean ± SE (n
541
= 3). Different letters above bars indicate significant difference at P<0.05 (Capital
542
letters denote significance within the same arsenic level at different doses of selenium;
543
lowcase letters denote significance within the same selenium level at different doses
544
of arsenic).
545
Fig.3. Effect of addition of As and Se in the solution on the uptake of As by flue-cured
546
tobacco after being grown for 14 days under hydroponic conditions. Symbols and
547
vertical lines in the curves are means and standard error of means. Each of the curves
548
was drawn based on the related single factor experiment. Fig 3A and 3B illustrate the
549
effects of As and Se on the uptake of As in the leaves and roots. Bars indicate
550
standard error of the mean. Different letters above bars indicate significant difference
551
at P<0.05 (Capital letters denote significance within the same arsenic level at different
552
doses of selenium; lowcase letters denote significance within the same selenium level
553
at different doses of arsenic).
554
Fig.4. Effect of addition of As and Se in the solution on the percentage of Se species
555
[SeCys, SeMet, Se(IV) and Se(VI)] in leaves (A) and roots (B) of flue-cured tobacco.
556
The Se species of leaves and roots treated with no selenium addition were not
557
detected.
558
Fig.5. Effect of addition of As and Se in the solution on the percentage of As species
559
[As(Ⅲ) and As(V)] in leaves (A) and roots (B) of flue-cured tobacco. The As species
560
of leaves and roots treated with no As addition were not detected.
561
Fig.6. Effect of addition of As and Se in the solution on the activities of SOD (A) and
562
POD (B) as well as GSH (C) and AsA (D) contents of flue-cured tobacco’s leaves. 21
563
The values are mean ± SE (n = 3). Different letters above bars indicate significant
564
difference at P<0.05 (Capital letters denote significance within the same arsenic level
565
at different doses of selenium; lowcase letters denote significance within the same
566
selenium level at different doses of arsenic.
567
Fig.7. Effect of addition of As and Se in the solution on MDA content of flue-cured
568
tobacco’s leaves. The values are mean ± SE (n = 3). Different letters above bars
569
indicate significant difference at P<0.05 (Capital letters denote significance within the
570
same arsenic level at different doses of selenium; lowcase letters denote significance
571
within the same selenium level at different doses of arsenic).
572 Fig 1
60
4
Shoot fresh weight (g plant-1)
A
a A a b B C
50
a a AA
B
Se0
a b A B
b B
a A
Se0.1
a AB
Se1 Se5
a ab B C
40 c C
a C
30 20
a A
3
a A b B
ab D
b D
a A a B
a D
2 a B
a C
1
10 0
0 As0
As1
As5
As0
As1
As treatments (mg L-1)
574 575
Root fresh weight (g plant-1)
573
As5
As treatments (mg L-1)
Fig. 2
576 577
Se content in leaves (mg kg-1)
A 10 8
a A
b A
a
a D
a C
a C a D
As1
300 200
a C
a C a D
400
100
c B
4 2
B
b B
b A
a B
b B
As0
578
c A
a B
Se0 Se0.1 Se1 Se5
6
0
b A
a A
B
20 b C
b C a
a C
Se content in roots (mg kg-1)
12
b C
C
0 As5
As treatments (mg L-1)
As0
As1
As5
As treatments (mg L-1)
22
579
Fig. 3
580
As content in leaves(mg kg-1)
Se 0 Se 0.1 Se 1 Se 5
15
a AB a
A
400
B a
a
B a
C
C a C
b b A A
b A
10
5 B
0
B
c
c Ac B B
As0
c C
As1
As5
c c c A B A
As0
As treatments (mg L-1)
581
300
100
b b b b A b AB AB B c
582
A
a
20
500
a
B
A
As content in roots (mg kg-1)
25
0 As1
As5
As treatments (mg L-1)
Fig.4
583
100
100
SeCys SeMet Se(IV) Se(VI)
80
60
60
40
40
20
20
0
0 s0 s1 s5 s0 s1 s5 s0 s1 s5 s0 s1 s5 0 A 0A 0A .1A .1A .1A 1A 1A 1A 5A 5 A 5A S e Se Se Se0 Se0 Se0 Se Se Se Se S e Se
584
Se(IV) and Se(VI)
Percentage of SeCys, SeMet, Se(IV) and Se(VI)
80
Percentage of SeCys, SeMet,
B
A
Treatments (mg kg-1)
s0 s1 s5 s0 s1 s5 s0 s1 s5 s0 s1 s5 0A 0A 0A .1A .1A .1A e1A e1A e1A e5A e5A e5A Se S e Se Se0 Se0 Se0 S S S S S S
Treatments (mg kg-1)
585 586 587 588 589 590 591 592 593 594 23
595
Fig.5
596
100
100 B
As(III) As(V)
80
80
60
60
40
40
20
20
0
598
0 s 0 s0 s0 s0 s1 s1 s1 s1 s 5 s5 s5 s5 0A 1A 1A 5A 0A 1A 1A 5A 0A 1A 1A 5A Se Se0. Se Se Se Se0. Se Se Se Se0. Se Se Treatments (mg kg-1)
597
Percentage of As(III) and As(V)
Percentage of As(III) and As(V)
A
s0 s0 s0 s0 s1 s1 s1 s1 s5 s5 s5 s5 0A 1A 1A 5A 0A 1A 1A 5A 0A 1A 1A 5A Se Se0. Se Se Se Se0. Se Se Se Se0. Se Se Treatments (mg kg-1)
Fig.6
599
500
a ab A A
Se0 Se0.1 Se1 Se5
400
a
b A
A
b B
a
C
A
a a b A b AB BC C
a b B C
a A
a a a A AB a B B
b D
POD activity (U g-1 min-1 FW-1 )
300 250
a B
200
300 150
a C
b B
c
200
C
100
b C
b D
100
50
0
0 a A
B
A
800
600
a A
D
a
a a A A
40
b A
400
a B
a B
a a B b C D c c C D
b b C C
ab b b b A A AB B
b b B BC c C
a a B B
30
20
10
200
0
0
As0
600
350
AsA content (ug g-1 FW-1 )
SOD activity (U g-1 FW-1 )
A
GSH content (ug g-1 FW-1)
600
As1 As treatments (mg L-1)
As5
As0
As1
As5
As treatments (mg L-1)
601 602 603 604 24
605
Fig. 7
6
4
a B
b A
-1
MDA content(nmol g )
5
a A
Se 0 Se 0.1 Se 1 Se 5 a C a D
b B
3
c A
b D
a C
a c Ba B B
2 1 0 As0
606
As1
As5
As treatments (mg L-1)
607
25
S0098-8472(15)00081-7 http://dx.doi.org/doi:10.1016/j.envexpbot.2015.04.008 EEB 2927
To appear in:
Environmental and Experimental Botany
Received date: Revised date: Accepted date:
15-11-2014 4-4-2015 14-4-2015
Please cite this article as: Han, Dan, Xiong, Shuanglian, Tu, Shuxin, Liu, Jinchang, Chen, Cheng, Interactive effects of selenium and arsenic on growth, antioxidant system, arsenic and selenium species of Nicotiana tabacum L.Environmental and Experimental Botany http://dx.doi.org/10.1016/j.envexpbot.2015.04.008 This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
1
Interactive effects of selenium and arsenic on growth, antioxidant system, arsenic and
2
selenium species of Nicotiana tabacum L.
3 4
First name: Dan; Family name: Hana, b, c
5
First name: Shuanglian; Family name: Xionga, b, c
6
First name: Shuxin; Family name: Tua, b, c
7
First name: Jinchang; Family name: Liua, b, c
8
First name: Cheng; Family name: Chena, b, c
9 10
a
11
430070, China
12
b
13
China
14
c
15
Yangtze River), Ministry of Agriculture, Wuhan 430070, China
College of Resources and Environment, Huazhong Agricultural University, Wuhan
Microelement Research Center, Huazhong Agricultural University, Wuhan 430070,
Key Laboratory of Arable Land Conservation (Middle and Lower Reaches of
16 17
Corresponding author
18
Shuanglian Xiong; College of Resources and Environment, Huazhong Agricultural
19
University, Wuhan 430070, China; Tel.: +86 027 87282137 fax: +86 027 87288618.
20
E-mail: [email protected] (S. Xiong).
21
Shuxin Tu; College of Resources and Environment, Huazhong Agricultural University,
22
Wuhan 430070, China. E-mail: [email protected] (S. Tu).
1
23
Highlights
24
●
The moderate dose of Se/As in solution promoted the growth of FCT.
25
●
Different Se/As levels in solution affects the ratios of Se/As species of FCT.
26
●
Se mitigates As toxicity by improving the antioxidant capacity.
27
●
Se mitigates As toxicity by influencing on the Se/As species of FCT changes.
28 29
Abstract
30
This paper is aimed to study separate and interactive effects of selenium (Se) (selenite,
31
0-5 mg L-1) and arsenic (As) (arsenate, 0-5 mg L-1) on the growth and the antioxidant
32
system of flue-cured tobacco (FCT) as well as the contents and species of As and Se
33
in FCT through a hydroponic experiment and clarify the possible mechanism how Se
34
alleviates the toxicity of As. The results were: single addition of Se (≤ 1 mg L-1) or As
35
(1 mg L-1) by a low dose could stimulate the growth of FCT, but the growth of FCT
36
would be inhibited when Se (5mg L-1) or As (5mg L-1) was added by a high dose. Low
37
As levels stimulated the uptake of Se but high levels of As posing the opposite effects
38
with the low Se dosage. However, the addition of As always inhibited the uptake of Se
39
with high Se levels. Moreover, Se showed dual effects on the uptake of As. At the low
40
As dose (1mg L-1), the addition of Se inhibited the growth of FCT, but significantly
41
promoted the activity of superoxide dismutase (SOD) and peroxidase (POD) enzymes
42
as well as the content of MDA. Meanwhile, the percentages of organic Se and As(III)
43
in the leaves of FCT declined with the increasing Se dose. However, the addition of
44
Se by a moderate dose (0.1mg L-1) alleviated the toxicity of the high As dose (5mg L-1 )
45
and promoted the growth of FCT by elevating the ability of anti-oxidative stress of
46
FCT and reducing the contents of MDA and As in FCT. The Se species in the leaves
47
of FCT existed in organic ones (SeCys and SeMet) (100%), while the major As
48
speciation was As(III) (75%). Likewise, the addition of As counteracted the toxicity of
49
high Se dose (5 mg L-1) and promoted the growth of FCT slightly as it reduced the
50
formation of organic Se or failed to transform excess inorganic Se species into organic
51
ones and depressed the contents of Se in the roots and leaves of FCT. In a word, the
52
low Se dose (0.1mg L-1) alleviated of the toxicity of the high As dose and the addition 2
53
of As counteracted the toxicity of high Se dose (5 mg L-1), as a result of which the
54
promotion of the growth of FCT were realized.
55 56
Keywords: Arsenate; Selenite; Interaction; Antioxidant system; Species.
57
Abbreviations: Se, selenium; As, arsenic; MDA, malondialdehyde; SOD, superoxide dismutase;
58
POD, peroxidase; AsA, ascorbate acid; GSH, glutathione; As(V),arsenate; As(III), arsenite; ROS,
59
reactive oxygen species; MMA, monomethylarsonicacid; DMA, dimethylarsinic acid; Cd,
60
cadmium; Hg, mercury; Ni, nickel; Pb, lead; GR, glutathione reductase; Se(IV), selenite; Se(VI),
61
selenate; SeCys, selenocysteine; SeMet, selenomethionine; AR, arsenate reductase; PC,
62
phytochelatins.
3
63
1. Introduction
64
Arsenic (As) is a severe pollutant which is highly toxic to animals and plants and
65
widely distributes in the environment. Arsenic exists in the forms of arsenate [As(V)],
66
arsenite [As(III)], monomethylarsonic acid [MMA] and dimethylarsinic acid [DMA],
67
but As(V) and As(III) are the main species (Tripathi et al., 2007; Zheng et al., 2013),
68
which mainly come from mining, coal ash, dust, off gas, pesticides and sewage
69
sluge(Meunier et al., 2011; Saunders et al., 2010). The accumulation of As in soil
70
doesn’t only can affect the growth and development of plants, but also pose a threat to
71
human health via the food chain. Arsenic impedes the photosynthesis and reduces the
72
contents of essential nutrients, thus inhibits the growth of crops and even causes them
73
death (Garg and Singla, 2011). For human, arsenic may lead to cancerous and
74
non-cancerous diseases, including bladder cancer, lung cancer, liver cancer and so on
75
(Farnese et al., 2014).
76
Although there is no evidence that selenium (Se) is an essential element for plants so
77
far, it is an essential microelement for human and animals. An appropriate dose of Se
78
can improve the antioxidant capacity, scavenge excessive oxygen free radicals,
79
decrease lipid peroxidation, defer senescence, promoting the growth of plants (Lin et
80
al., 2012), and detoxify heavy metals (metalloids) in plants, for example arsenic (As)
81
(Malik et al., 2012), cadmium (Cd)(Feng et al., 2012; Lin et al., 2012; Saidi et al.,
82
2014), mercury (Hg) (Zhang et al., 2012a), nickel (Ni) (Gajewska et al., 2013) and
83
lead (Pb) (Mroczek-Zdyrska and Wojcik, 2012). Currently, the researches on the
84
mechanism how Se mitigates the toxicity of As are mainly concentrated on the
85
elimination of reactive oxygen species (ROS), the suppression of lipid peroxidation
86
and the enhancement of the antioxidant capacity of plants(Kramárová et al., 2012;
87
Malik et al., 2012). Se exists mainly in the forms of Se(IV), selenate Se (VI),
88
selenocysteine (SeCys) and selenomethionine (SeMet) in plants (Zhu et al., 2009).
89
After absorbed by plants, Se(IV) or Se(VI) is converted into other forms like
90
selenocysteine (SeCys) and selenomethionine (SeMet) (Zhu et al., 2009). Moreover, 4
91
Se can replace sulphur in the amino acids as SeMet and SeCys due to their
92
physicochemical similarity. And the organic Se species (SeCys and SeMet) can be
93
incorporated into proteins, replacing cysteine (Cys) and methionine (Met),
94
respectively, which can result in toxicity in plants (Navarro-Alarcon and
95
Cabrera-Vique, 2008; White et al., 2004). However, the toxicity of soluble inorganic
96
As is greater than that of organic As, and the toxicity of As(III) is higher than that of
97
As(V) in the environment (Yamauchi, 1994; Yin et al., 2013). Having taken up by the
98
roots of plants via the phosphate transport pathway (Wu et al., 2011b; Zhao et al.,
99
2010), As(V) can be rapidly reduced to As (III) by arsenate reductase (AR) (Zhao et
100
al., 2009). As(III), which can also be taken up by the roots of plants mainly through
101
silicic acid transport protein (Ma et al., 2008), is chelated with polypeptides like GSH
102
and PCs and finally stored in the vacuoles of roots to detoxify As(Liu et al., 2010; Ye
103
et al., 2011; Zhang et al., 2012c). A previous study showed that Se could mitigate the
104
toxicity of As via antagonistic effects in Pteris vittata (Feng et al., 2009).
105
However, the changes of As and Se species in plants under the exposure of As and Se
106
are still unclear. We infer that Se can mitigate the toxicity of As by regulating the
107
antioxidant system and simultaneously affecting As species in plants.
108
Tobacco leaf, which contains abundant and high-quality soluble proteins (Teng and
109
Wang, 2012), is considered as an ideal material to produce Se-rich protein. In this
110
study, Nicotiana tabacum L. was chosen as the test material to investigate: (1) the
111
responses of the growth and antioxidant systems of FCT to different doses of Se and
112
As; (2) the relation among the variations of As species and the detoxification of As
113
after Se supplementation.
114
2. Materials and methods
115
2.1. Seedling cultivation
116
The cultivar was N. tabacum K326, and the floating cultivation method was adopted
117
for the cultivation of seedlings. Later, the seedlings of similar sizes were transplanted 5
118
into plastic pots containing 10 L nutrient solution which was composed of 4 mmolL-1
119
Ca(NO3)2·4H2O, 5 mmolL-1 KNO3, 1mmolL-1 NH4H2PO4, 2 mmolL-1 MgSO4·7H2O,
120
0.01 mmolL-1 EDTA-Fe, 0.046 mmolL-1 H3BO3, 0.0008 mmolL-1 ZnSO4·7H2O and
121
0.0003 mmolL-1 CuSO4·5H2O. The plants grew in a greenhouse with natural light at
122
25-30℃.
123
2.2. Experimental design and implementation
124
A hydroponic experiment of four Se levels, i.e. 0, 0.1, 1.0 and 5.0 mg L-1, and three
125
As levels, i.e. 0, 1.0 and 5.0 mg L-1, was designed. As and Se were added in the forms
126
of Na3AsO4.12H2O and Na2SeO3, respectively. A randomized complete block design
127
was employed. There was a total of 12 treatments, namely CK (without the addition
128
of Se and As), Se0.1As0, Se1As0, Se5As0, Se0As1, Se0.1As1, Se1As1, Se5As1,
129
Se0As5, Se0.1As5, Se1As5 and Se5As5, and each treatment was repeated for three
130
times.
131
Four-leaf FCT seedlings were transplanted to 1/4 strength Hoagland-Arnon nutrient
132
solution at first and three days later, the solution was replaced by 1/2 strength nutrient
133
and the nutrient solution was renewed every five days. After forty days, the seedlings
134
of even size were transplanted to the plastic cases (22×16×7cm) and subject to the
135
above-mentioned Se and/or As treatments with full strength Arnon-Hoagland nutrient
136
solution, and each pot contained 2 plants. The plants were harvested after fourteen
137
days. After rinsed carefully with tap water and deionized water successively, the
138
separated fresh leaves and roots were weighed and divided into two parts. One was
139
immersed in N2 liquid immediately and stored at -80℃ to determine the Se and As
140
species and the indices of the antioxidant systems later. The other was over-dried at
141
105°C for 15 min to de-enzyme at first, and then at 65°C for 48 h and finally
142
pulverized to determine the contents of As and Se.
6
143
2.3. Determination of Se and As contents and species
144
The contents of Se and As were determined with a hydride generation atomic
145
fluorescence spectrometer (AFS8220, Beijing Titan Instruments Co., China) (Feng et
146
al., 2009a) after the tissues of FCT were digested with concentrated HNO3-HClO4.
147
The accuracy of elemental analysis was verified by standard reference materials
148
[GBWO7602 (GSV-1)] from the Center for Standard Reference of China.
149
A methanol: water (1:2) method was used to extract Se species in leaves or roots of
150
FCT plants. The separation of SeIV, SeVI, SeMet and SeCys in the green parts of FCT
151
was carried out with a anion exchange chromatography in which the column was
152
connected to a ultraviolet treatment-hydride generation atomic fluorescence
153
spectrometry (UV-HG-AFS) detection system (Han et al., 2013) online.
154
The extraction of As species was similar to that of Se species. Because no organic
155
arsenic in FCT were detected in a preliminary experiment, only As(V) and As(III)
156
were measured in this study. The separation of As(V) and As(III) in leaves and roots
157
of FCT plants was conducted with the anion exchange chromatography in which the
158
column was also connected to the HG-AFS detection system (Zhang et al., 2002)
159
online.
160
The HPLC system consisted of a SHIMADZU 10ATvp Plus liquid chromatography
161
pump (SHIMADZU, Tokyo, Japan), a Rheodyne 7725i injector (Rheodyne, Cotati,
162
USA) and a Hamilton PRP-X100 column (Hamilton, Reno, NV). The mobile phase
163
for HPLC was 15 mmol L-1(NH4)2HPO4 (pH 6.0, 1.0 mL min-1). As for the HG phase,
164
the reduction agents were 1.5% KBH4 (m/v)+0.5% KOH (m/v) and the carrier
165
solution was 7% HCl (v/v). The detection phase was AFS8220, with the Se hollow
166
cathode lamp current (General Research Institute for Nonferrous Metals, Beijing,
167
China) of 50 mA, the negative high voltage of photomultiplier tube of 270V, the flow
168
rate of carrier gas of 400 mL min-1 and the flow rate of makeup gas of 600 mL min-1.
7
169
2.4. Assay of enzymatic and non-enzymatic antioxidants
170
The activity of superoxide dismutase (SOD) was determined with the method put
171
forward by Zhang et al.(Zhang et al., 2012b). In brief, 0.5g fresh FCT leaves was
172
grounded in 5mL extraction buffer containing 50 mM potassium phosphate (pH7.8) at
173
first, and then the homogenate was centrifuged at 10,000×g for 15 min at 4°C. 3mL
174
reaction mixture contained 13 mM methionine, 75 μM NBT, 2 μM riboflavin, 0.1 mM
175
EDTA and 100μL enzyme extract. The reaction mixture was illuminated for 15 min.
176
The sample absorbance was determined at 560 nm, and the unit SOD activity was
177
defined as the amount of enzyme to inhibit 50% of the NBT reduction.
178
The activity of peroxidase (POD) was measured with the method described by Zhang
179
et al. (Zhang et al., 2012b). In brief, 0.5g fresh leaves of FCT were extracted with 5
180
mL 50mM potassium phosphate buffer (pH 5.5). Afterwards, the extracts were
181
centrifuged at 10,000×g for 15min at 4°C. The reaction mixture contained 1 mL
182
extraction buffer, 5μL 30% H2O2, 5μL guaiacol and 15μL supernatant. The molar
183
extinction coefficient of 26.6 mM−1cm−1 was used for the calculation of the enzyme
184
activity.
185
Ascorbate (AsA) was extracted from 0.5g FCT leaves with 10g L−1 oxalic acid and
186
determined spectrophotometrically with 2,4-dinitrophenylhydrazine colorimetry
187
method proposed by Zhang et al. (Zhang et al., 2012b). 0.5g samples were
188
homogenized with 3% metaphosphoric acid at first, then the homogenate was
189
centrifuged for 10min at 10,000×g and finally the supernatant was used for
190
glutathione (GSH) assays (Zhang et al., 2012b).
191
The MDA content was assayed with 2.5 mL solution of 20% (w/v) trichloroacetic acid,
192
which included 0.5% (w/v) thiobarbituric acid and 1.5 mL enzyme extract. The
193
solution was kept in boiling water for 20min bath at first and then cooled quickly.
194
After refrigeration, the homogenate was centrifuged at 5,000 g for 10 min at 25°C.
195
The absorbances of supernatant were recorded at 532 nm and 600 nm, respectively.
196
The absorbance at 600 nm was subtracted from that at 532 nm. The MDA content was
197
calculated based on the extinction coefficient of MDA, namely 155 mM−1cm−1(Feng 8
198
et al., 2009b).
199
2.5. Statistical analysis
200
All data were subject to two-way ANOVA analysis and Tukey's multi-comparisons
201
test (P≤0.05). The results were expressed as the means and the corresponding standard
202
errors. All statistical analyses were completed using the SAS 8.1 software.
203
3. Results
204
3.1. Growth of FCT
205
Without the addition of As, low Se levels (≤ 1mg L-1Se) stimulated the growth of FCT,
206
but high Se levels (5 mg L-1) had the opposite effects on and inhibited the growth of
207
FCT compared with the CK treatment (Fig. 1AB). The fresh weights of leaves and
208
roots of FCT in Se5As0 treatment were 32% and 43% of those of the CK treatment,
209
respectively (Fig. 1AB). Similarly, in the absence of Se, 1mg L-1 As stimulated the
210
growth of FCT, but 5mg L-1As significantly hindered the growth of FCT, especially
211
the roots of FCT (Fig. 1AB). The fresh weights of leaves and roots of FCT in Se0As1
212
treatment were 22% and 24% higher than those in the CK treatment, respectively. The
213
fresh weight of roots in Se0As5 treatment was 24% lower than that in the CK
214
treatment (Fig. 1AB).
215
Under low As treatments (1 mg L-1 As), the addition of Se inhibited the growth of FCT
216
(Fig. 1AB). The fresh weights in Se0.1As1, Se1As1 and Se5As1 treatments were 91%,
217
68%, 38% (for leaves) and 88%, 108%, 35% (for roots) of those in Se0As1 treatment,
218
respectively. However, at the high As level (5mg L-1), the low Se level (0.1mg L-1Se)
219
enhanced but high Se level (5mg L-1Se) obviously depressed the growth of FCT (Fig.
220
1AB). For example, the fresh weights of shoots and roots in Se0.1As5 treatment were
221
1.1 times and 1.5 times of those in Se0As5 treatment, respectively. Nevertheless, the
222
fresh weights of shoots and roots in Se5As5 treatment were 40% and 75% of those in
9
223
Se0As5 treatment, respectively (Fig. 1AB).
224
3.2. Uptake, distribution and species of Se or As of FCT
225
At a certain As dose, the contents of Se in the leaves and roots of FCT went up along
226
with the increasing Se level (Fig. 2AB).
227
Se and As had significant interactive effects on the contents of Se in leaves and roots
228
of FCT (F=79.26 and 81.06, P<0.01, respectively). The effects of As on the uptake of
229
Se depended on the levels of Se and As in solution. At the low Se level (≤ 1 mg L-1), 1
230
mg L-1 As promoted the uptake of Se by the leaves and roots of FCT, but 5 mg L-1As
231
had negative effects on the uptake of Se.
232
At the high Se level (5 mg L-1), As showed antagonistic effects on the uptake of Se in
233
the leaves and roots of FCT. The contents of Se in the leaves and roots of FCT in
234
Se5As1 and Se5As5 treatments were 82% and 69% (for roots), 66% and 61% (for
235
leaves) of those in Se5As0 treatment, respectively (Fig. 2AB).
236
At a certain Se level, the contents of As in the leaves and roots of FCT increased
237
along with elevation of the As level significantly (Fig. 3AB), and in particular the
238
content of As in roots was far higher than that in the leaves (Fig. 3AB).
239
The interaction of Se and As had significant effects on the uptake of As by FCT
240
(F=34.57 and 26.63, P<0.01, respectively). At 1 mg L-1 As level, the elevation of the
241
Se levels raised the As content in the leaves (Fig. 3A) but failed to enhance the As
242
content in the roots of FCT. However, at 5 mg L-1 As level, the growth of Se level
243
remarkably reduced the contents of As in leaves and roots of FCT (Fig. 3AB).
244
Only SeCys and Se(IV) were detected in the roots, whereas SeCys, SeMet and Se(IV)
245
were observed in the leaves of FCT (Fig. 4AB). In 0.1 mg L-1 Se treatment, main Se
246
species in the leaves of FCT were organic ones (SeCys and SeMet) (58%-100%),
247
which gradually increased with the growth of the As level (Fig. 4A). Similarly, the
248
proportion of organic Se species (SeCys) in the roots of FCT went up from 30% to
249
69% with the growth of the As level (Fig. 4B).
250
In 1 mg L-1 Se treatment, the percentage of organic Se species declined in the leaves 10
251
but increased in the roots of FCT along with the elevation of the As level. To be
252
specific, the proportions of organic Se species (SeCys and SeMet) in the leaves
253
decreased from 68% (Se1As1) to 42% (Se1As5), while the percentage of organic Se
254
species (SeCys) in the roots of FCT went up from 47% (Se1As1) to 84% (Se1As5).
255
In 5 mg L-1 Se treatment, the percentages of organic Se species in the leaves and roots
256
of FCT decreased along with the elevation of the As level.
257
In the leaves of FCT, As (V) was the main speciation at the low As level of 1mg L-1
258
(63%-94%), whereas As(III) was the major As speciation at the high As level of 5mg
259
L-1 (63%-78%) (Fig.5A). At a certain As level, the proportion of As(III) in the leaves
260
of FCT declined along with the growth of the Se level. For example, the proportion of
261
As(III) in the leaves dropped from 37% to 6% at 1mg L-1 As but decreased from 74%
262
to 63% at 5mg L-1 As along with the elevation of the Se level.
263
As(III) was the main As speciation in the roots of FCT (Fig. 5B). At the low As level
264
(1mg L-1), 0.1mg L-1 Se reduced the proportion of As(III) in the roots of FCT but the
265
other Se levels raised the proportion of As(III) in comparison with the Se0As1
266
treatment. At the high As level (5mg L-1), the elevation of the Se level had no
267
significant effects on the proportions of As(III) and As (V) (Fig. 5B).
268
3.3. Antioxidant system of FCT under As/Se stress
269
Se and As treatments had great influences on the activities of SOD and POD (P<0.01).
270
Regardless of the addition of As, the addition of Se markedly increased the activities
271
of SOD and POD of the leaves of FCT (Fig. 6AB, P<0.05). However, whether Se is
272
added into the solution or not, the elevation of the As level significantly enhanced the
273
SOD activity but generally decreased the POD activity of the leaves of FCT except
274
that the POD activity was significantly enhanced at the Se level of 1 mg L-1 and along
275
with the growth of the As level (Fig. 6AB).
276
As and Se had significant influences on the GSH content in the leaves of FCT
277
(F=15.50, P<0.01). Without the addition of As in the solution, the growth of the Se
278
level significantly enhanced the GSH content in the leaves of FCT (Fig. 6C). 11
279
At a low As level of 1 mg L-1, the GSH content was also enhanced by increasing the
280
Se level except for the GSH content was reduced by 15% at the Se level of 1 mg L-1
281
compared with the Se0As1 treatment (Fig.6C). At the high As level of 5 mg L-1, the
282
GSH content did not significantly change with the increasing Se level (Fig. 6C).
283
When Se was not added in the solution, the increase of the As level significantly
284
enhanced the GSH content in the leaves of FCT. However, when Se was present in the
285
solution, the addition of As appeared to show insignificant effects on or reduce the
286
GSH content in FCT (Fig. 6C).
287
The interaction of Se and As significantly affected the AsA content in the leaves of
288
FCT (F=60.07, P<0.01). At a certain As level, the increasing Se levels significantly
289
raised the AsA content in the leaves of FCT. When no Se or 0.1 mg L-1 Se was added
290
in the solution, 1 mg L-1 As reduced but 5 mg L-1 As recovered or increased the AsA
291
content compared with the CK and Se0.1As0 treatments, respectively (Fig. 6D).
292
However, when 1 or 5 mg L-1 Se was added in the solution, 5 mg L-1 As significantly
293
enhanced the AsA content (Fig. 6D).
294
Se and As treatments could dramatically affect the MDA content (P<0.01). When no
295
As was added in the solution, 0.1 mg L-1 Se significantly reduced the MDA content in
296
the leaves of FCT but 1 and 5 mg L-1 Se enhanced the MDA content compared with
297
the CK treatment (Fig. 7). However, when Se was absent from the solution, 1 mg L-1
298
As reduced the MDA content in the leaves of FCT but 5 mg L-1 As resulted in the
299
reduction of the MDA content to the level in the CK treatment (Fig. 7).
300
When 1 mg L-1 As was added into the solution, the increasing Se level significantly
301
enhanced the MDA content in the leaves of FCT. However, with 5 mg L-1 As in the
302
solution, only 5 mg L-1 Se significantly enhanced the MDA content. In the presence of
303
0.1 mg L-1 Se in the solution, the addition of As did not significantly affect the MDA
304
content in FCT. However, when 1 or 5 mg L-1 Se was added in the solution, 1 mg L-1
305
As significantly enhanced but 5 mg L-1 significantly reduced the MDA content in the
306
leaves of FCT.
12
307
4. Discussion
308
This study attempted to illuminate the mechanism how Se detoxifies As via regulating
309
the antioxidant systems of FCT and the variations of species of As and Se in FCT. As
310
expected, the addition of Se can detoxify As, showing as the stimulated leaf and root
311
biomass of FCT exposed to high levels of As. However, this alleviation process might
312
be dependent on the dosages of Se and As, because the high Se level (5 mg L-1) had
313
already showed toxic effects on the plant growth whether As was added into the
314
solution or not. Furthermore, when plants were exposed to 1 mg L-1 As, the addition
315
of Se did not show beneficial but negative effects on the growth of FCT because the
316
addition of Se might counteract the beneficial effects of low As dosages on the growth
317
of FCT. Similar results have been reported by Malik et al. (2012) on mung bean
318
(Phaseolus aureus Roxb.) and Zhao et al. (2013b) on garlic (Allium sativum). With
319
increase in arsenic (As) concentration, a marked inhibition in the growth of plants was
320
observed. The plants treated 10 uM As (0.7 mg L-1) and supplemented with 2.5uM Se
321
(0.2 mg L-1) showed 22% growth improvement in shoots and 16% in roots compared
322
to those growing in As alone(Malik et al., 2012). Low-level exposure to Se(≤0.1 mg
323
L-1) or Hg (≤0.01 mg L-1) is beneficial for garlic growth, whereas Se(>1 mg L-1) or
324
Hg (>0.1 mg L-1) levels above certain threshold limits can be harmful. As for Se-Hg
325
co-exposed garlic, the stimulation of garlic growth by low levels of Se is also
326
enhanced by HgCl2 at low levels (≤0.1 mg L-1 Hg), by contrast, an antagonistic effect
327
between low levels of Se and higher Hg levels (1 mg L-1 or 10 mg L-1) is
328
observed(Zhao et al., 2013b).
329
Like the effects of As and Se of different levels on the growth of plant, the Se uptake
330
might also depend on the levels of As and Se in the solution. Low As levels stimulated
331
the uptake of Se but high levels of As appeared to bring about the opposite effects
332
when the plants were subject to low dosages of Se. However, when plants were
333
exposed to high Se levels, the addition of As always inhibited the uptake of Se.
334
Similar results about the uptake of As on Se have been reported on P. vittata (Feng et
13
335
al., 2009a) and garlic (Allium sativum) (Zhao et al., 2013a). The increased Se uptake
336
in FCT might be used to synthesize some important substances, such as GSH-Px
337
(glutathione peroxidase), and rebalance the excessive ROS, during which GSH will be
338
needed in huge doses, like the significant growth of the GSH content in this study (Fig.
339
6C). However, when As and Se was added in excess, some vital substances (for
340
example GSH) might not satisfy the metabolism demands of As and Se. Therefore,
341
there was a competition between As and Se to integrate with GSH, and they showed
342
the mutually antagonistic effects. The results above matched well with the hypothesis
343
of Feng et al. (2013). Interestingly, Se showed dual effects on the uptake of As in this
344
study. The exact reasons behind the stimulation of the As uptake in the leaves of FCT
345
subject to low As doses by Se were unknown (Fig. 3A). However, similar inhibition
346
effects of Se on the uptake of As were also reported on Phaseolus aureus Roxb.
347
(Malik et al., 2012) and Pteris vittata (Feng et al., 2009a). Se (SeO32- or SeO42-) at
348
high exposure levels (>1mg L-1) also significantly inhibited the uptake of Hg in
349
garlic when Hg2+ levels were higher than 1mg L-1 in the culture media (Zhao et al.,
350
2013a). Since As(V) and Se(IV) were taken up by roots via the phosphate transport
351
pathway(Wu et al., 2011a; Zhu et al., 2009), the antagonistic effects between Se and
352
As on their mutual uptakes might be related to their competition for binding sites.
353
The detoxification of As by Se might be also closely with the changes of As and Se
354
species. In the leaves of FCT, the addition of Se resulted in more accumulation of
355
As(V) and less accumulation of As(III) (Fig. 5A), but the opposite trends were
356
observed in the roots (Fig. 5B). It is well established that As(III) is more toxic than
357
As(V) in plants. Therefore, a conclusion could be drawn that Se could reduce the
358
toxicity of As since it reduced the transfer of As(III) from the roots to the
359
above-ground parts of plants.
360
When Se was added at low levels in the solution, organic Se species (SeCys and
361
SeMet) were predominant in the leaves of FCT, and the increasing As levels enhanced
362
the transformation of inorganic Se into organic Se (Fig. 4A), which might be related
363
with the antioxidative effects of low Se dosages (Feng et al., 2013). It was reported
364
that organic Se could directly quench ROS, especially hydroxylic free radical (OH•) 14
365
(Feng et al., 2013). Therefore, the enhancement of organic Se in the leaves of FCT
366
was conducive to the rebalance of ROS of plants. However, the proportion of
367
inorganic Se [Se(IV)] increased when FCT was subjected to the high levels of As and
368
Se. Se was considered as a pro-oxidant at high levels, and synthesized proteins in
369
place of S(Feng et al., 2013; Terry et al., 2000). Therefore, the more accumulation of
370
inorganic Se after the addition of high levels of Se and As might suggest that to avoid
371
the toxicity of high levels Se, plant will reduce the formation of organic Se or cannot
372
transform excess inorganic Se into organic over a short period of time. In addition, the
373
competition between As and Se to integrate with GSH might also a key influential
374
factor to the formation of organic Se, which was realized with the help of GSH (Feng
375
et al., 2013). Similar results have been reported by Han et al. (2013) on Nicotiana
376
tabacum L.. In the leaves and roots of FCT, the addition of Se resulted in more
377
accumulation of organic Se species at low Se levels and more accumulation of
378
inorganic Se species at high Se levels(Han et al., 2013). Moreover, Compared with
379
roots, shoots of all the three plants (alfalfa, maize, and soybean) had a higher
380
percentage of organic Se (especially SeCys) by using Se(IV)-spiked soil(Yu et al.,
381
2011).
382
As expected, Se could affect the antioxidant system and regulate the toxicity of As,
383
judged from the increased activities of SOD and POD and the enhanced contents of
384
GSH and AsA, suggesting that these antioxidants play important roles in the
385
detoxification of As by Se. However, Se also showed toxicity to FCT, as it increase
386
the MDA content (Fig.7), decreased the fresh weights of leaves and roots at high Se
387
levels (Fig.1AB). In line with the increased fresh weight of leaves (Fig.1A), the
388
decreased Se contents in the leaves and roots (Fig.2AB) and organic Se proportion
389
(Fig.4AB) as well as the enhanced SOD activity and contents of GSH and AsA, the
390
addition of As seemed to exert detoxification effects on the high Se level (5 mg L-1)
391
(Fig.4ACD).
15
392
5. Conclusion
393
The low Se level (0.1mg L-1Se) alleviated the toxicity of high As level (5 mg L-1) and
394
thus promoted the growth of FCT by regulating the antioxidant system and reducing
395
the transfer of As(III) from the roots to the above-ground parts of FCT. Likewise, the
396
addition of As counteracted the toxicity of high Se level (5 mg L-1) and promoted the
397
growth of FCT slightly because it reduced the formation of organic Se, failed to
398
transform excess inorganic Se into organic Se over a short period of time and
399
depressed the Se contents in roots and leaves of FCT.
400
Acknowledgments
401
This research was partially supported by National Science Foundation of China
402
(41101464) and National Special Fund for Agro-scientific Research in the Public
403
Interest (201303106).
404
405
406
407
408
409
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519 520 521 522 523 524 525 526 527 528 529 530 531 532 20
533
Fig.1. The biomass in shoots (A) and roots (B) of flue-cured tobacco treated with As
534
and Se for 14 days under hydroponic conditions. The values are mean ± SE (n = 3).
535
Different letters above bars indicate significant difference at P<0.05 (Capital letters
536
denote significance within the same arsenic level at different doses of selenium;
537
lowcase letters denote significance within the same selenium level at different doses
538
of arsenic).
539
Fig.2. The Se concentration in leaves (A) and roots (B) of flue-cured tobacco treated
540
with As and Se for 14 days under hydroponic conditions. The values are mean ± SE (n
541
= 3). Different letters above bars indicate significant difference at P<0.05 (Capital
542
letters denote significance within the same arsenic level at different doses of selenium;
543
lowcase letters denote significance within the same selenium level at different doses
544
of arsenic).
545
Fig.3. Effect of addition of As and Se in the solution on the uptake of As by flue-cured
546
tobacco after being grown for 14 days under hydroponic conditions. Symbols and
547
vertical lines in the curves are means and standard error of means. Each of the curves
548
was drawn based on the related single factor experiment. Fig 3A and 3B illustrate the
549
effects of As and Se on the uptake of As in the leaves and roots. Bars indicate
550
standard error of the mean. Different letters above bars indicate significant difference
551
at P<0.05 (Capital letters denote significance within the same arsenic level at different
552
doses of selenium; lowcase letters denote significance within the same selenium level
553
at different doses of arsenic).
554
Fig.4. Effect of addition of As and Se in the solution on the percentage of Se species
555
[SeCys, SeMet, Se(IV) and Se(VI)] in leaves (A) and roots (B) of flue-cured tobacco.
556
The Se species of leaves and roots treated with no selenium addition were not
557
detected.
558
Fig.5. Effect of addition of As and Se in the solution on the percentage of As species
559
[As(Ⅲ) and As(V)] in leaves (A) and roots (B) of flue-cured tobacco. The As species
560
of leaves and roots treated with no As addition were not detected.
561
Fig.6. Effect of addition of As and Se in the solution on the activities of SOD (A) and
562
POD (B) as well as GSH (C) and AsA (D) contents of flue-cured tobacco’s leaves. 21
563
The values are mean ± SE (n = 3). Different letters above bars indicate significant
564
difference at P<0.05 (Capital letters denote significance within the same arsenic level
565
at different doses of selenium; lowcase letters denote significance within the same
566
selenium level at different doses of arsenic.
567
Fig.7. Effect of addition of As and Se in the solution on MDA content of flue-cured
568
tobacco’s leaves. The values are mean ± SE (n = 3). Different letters above bars
569
indicate significant difference at P<0.05 (Capital letters denote significance within the
570
same arsenic level at different doses of selenium; lowcase letters denote significance
571
within the same selenium level at different doses of arsenic).
572 Fig 1
60
4
Shoot fresh weight (g plant-1)
A
a A a b B C
50
a a AA
B
Se0
a b A B
b B
a A
Se0.1
a AB
Se1 Se5
a ab B C
40 c C
a C
30 20
a A
3
a A b B
ab D
b D
a A a B
a D
2 a B
a C
1
10 0
0 As0
As1
As5
As0
As1
As treatments (mg L-1)
574 575
Root fresh weight (g plant-1)
573
As5
As treatments (mg L-1)
Fig. 2
576 577
Se content in leaves (mg kg-1)
A 10 8
a A
b A
a
a D
a C
a C a D
As1
300 200
a C
a C a D
400
100
c B
4 2
B
b B
b A
a B
b B
As0
578
c A
a B
Se0 Se0.1 Se1 Se5
6
0
b A
a A
B
20 b C
b C a
a C
Se content in roots (mg kg-1)
12
b C
C
0 As5
As treatments (mg L-1)
As0
As1
As5
As treatments (mg L-1)
22
579
Fig. 3
580
As content in leaves(mg kg-1)
Se 0 Se 0.1 Se 1 Se 5
15
a AB a
A
400
B a
a
B a
C
C a C
b b A A
b A
10
5 B
0
B
c
c Ac B B
As0
c C
As1
As5
c c c A B A
As0
As treatments (mg L-1)
581
300
100
b b b b A b AB AB B c
582
A
a
20
500
a
B
A
As content in roots (mg kg-1)
25
0 As1
As5
As treatments (mg L-1)
Fig.4
583
100
100
SeCys SeMet Se(IV) Se(VI)
80
60
60
40
40
20
20
0
0 s0 s1 s5 s0 s1 s5 s0 s1 s5 s0 s1 s5 0 A 0A 0A .1A .1A .1A 1A 1A 1A 5A 5 A 5A S e Se Se Se0 Se0 Se0 Se Se Se Se S e Se
584
Se(IV) and Se(VI)
Percentage of SeCys, SeMet, Se(IV) and Se(VI)
80
Percentage of SeCys, SeMet,
B
A
Treatments (mg kg-1)
s0 s1 s5 s0 s1 s5 s0 s1 s5 s0 s1 s5 0A 0A 0A .1A .1A .1A e1A e1A e1A e5A e5A e5A Se S e Se Se0 Se0 Se0 S S S S S S
Treatments (mg kg-1)
585 586 587 588 589 590 591 592 593 594 23
595
Fig.5
596
100
100 B
As(III) As(V)
80
80
60
60
40
40
20
20
0
598
0 s 0 s0 s0 s0 s1 s1 s1 s1 s 5 s5 s5 s5 0A 1A 1A 5A 0A 1A 1A 5A 0A 1A 1A 5A Se Se0. Se Se Se Se0. Se Se Se Se0. Se Se Treatments (mg kg-1)
597
Percentage of As(III) and As(V)
Percentage of As(III) and As(V)
A
s0 s0 s0 s0 s1 s1 s1 s1 s5 s5 s5 s5 0A 1A 1A 5A 0A 1A 1A 5A 0A 1A 1A 5A Se Se0. Se Se Se Se0. Se Se Se Se0. Se Se Treatments (mg kg-1)
Fig.6
599
500
a ab A A
Se0 Se0.1 Se1 Se5
400
a
b A
A
b B
a
C
A
a a b A b AB BC C
a b B C
a A
a a a A AB a B B
b D
POD activity (U g-1 min-1 FW-1 )
300 250
a B
200
300 150
a C
b B
c
200
C
100
b C
b D
100
50
0
0 a A
B
A
800
600
a A
D
a
a a A A
40
b A
400
a B
a B
a a B b C D c c C D
b b C C
ab b b b A A AB B
b b B BC c C
a a B B
30
20
10
200
0
0
As0
600
350
AsA content (ug g-1 FW-1 )
SOD activity (U g-1 FW-1 )
A
GSH content (ug g-1 FW-1)
600
As1 As treatments (mg L-1)
As5
As0
As1
As5
As treatments (mg L-1)
601 602 603 604 24
605
Fig. 7
6
4
a B
b A
-1
MDA content(nmol g )
5
a A
Se 0 Se 0.1 Se 1 Se 5 a C a D
b B
3
c A
b D
a C
a c Ba B B
2 1 0 As0
606
As1
As5
As treatments (mg L-1)
607
25