He—Ne激光对小麦幼苗增强UV—B辐射损伤的修复效应

采用 He- Ne激光辐照对增强 UV- B辐射后小麦幼苗的损伤修复作用进行了研究。小麦种子在盛有湿滤纸的培养皿内 2 5℃下进行萌发。萌发后小麦幼苗在光合有效辐射 (PAR)为 2 2 0 μmol· m- 2 · S- 1的光背景下 ,经 1 0 .0 8k J·m- 2 · d- 1的增强 UV- B辐射 ,然后再用 5m W· mm- 2的 He- Ne激光进行辐照。通过小麦幼苗丙二醛 (MDA)、抗坏血酸 (As A)、超氧化物歧化酶 (SOD)和紫外吸收物含量及活性的变化 ,测定了 He- Ne激光对小麦 UV- B损伤修复的作用。结果显示 ,MDA、SOD、As A和紫外吸收物的变化同小麦幼苗损伤修复的能力相关联。He- Ne激光辐照可使 UV- B辐射后小麦幼苗 MDA的含量明显减少、As A含量明显增加、SOD活性增强及紫外吸收物含量显著增加。说明增强 UV- B对小麦幼苗生理水平的辐射损伤 ,能够被一定剂量的 He- Ne激光辐照而得到部分修复。但是 ,采用同等波长和功率的红光照射 ,其 MDA、SOD、As A和紫外吸收物均无明显变化 ,证明激光的促进修复作用并非由激光的光效应所致     

增强UV—B辐射和CO2复合作用对蚕豆幼苗生长和光合作用的影响

在4.52 kJ*m-2*d-1 UV-BBE的UV-B辐射和700 μmol*mol-1的CO2浓度人工模拟复合处理下,研究了对蚕豆(Vicia faba L.)幼苗的生长和光合作用的影响.结果表明,UV-B辐射单因子明显降低蚕豆幼苗的株高、叶面积和生物量,CO2单因子的作用正好相反,二者的作用程度随着处理时间的延长而增大.UV-B辐射和CO2复合作用对蚕豆幼苗的生长影响不明显.同时,增强的UV-B辐射单因子还使蚕豆幼苗的光合速率、气孔导度和水分利用率下降,CO2单因子的作用也相反,且CO2单因子的促进程度大于UV-B辐射单因子的抑制程度.而在UV-B辐射和CO2复合作用下,蚕豆幼苗的光合作用参数基本与对照同步.分析认为,UV-B辐射和CO2复合作用对蚕豆幼苗的影响是一种拮抗作用.     

聚γ—谷氨酸生产菌地衣芽孢杆菌的He—Ne激光辐射效应

应用He Ne激光对聚γ 谷氨酸生产菌地衣芽孢杆菌BacilluslicheniformisATCC9945A进行辐射处理。研究了不同剂量激光辐射对菌体生长的影响 ,0 .48mw·cm-2 、15min的剂量利于菌体的诱变。 2种激光辐射方式中 ,“生理盐水菌悬液”辐射方式诱变效果较好。延滞期的菌体细胞对激光辐射最敏感 ,随着菌体培养进程 ,其激光辐射抗性逐渐增强。另外 ,发现菌体的芽孢对激光辐射不敏感。经聚γ 谷氨酸发酵试验和菌体扫描电镜观察 ,发现He Ne激光对地衣芽孢杆菌具有明显的生物刺激效应和诱变作用 ,并初步筛选到产聚γ 谷氨酸含量有较大变化的辐射变异菌株 ;同时 ,通过对变异菌株的细胞外、胞周间、细胞内三位区的PGA、RNA、DNA分析和发酵过程检测 ,进一步证实了He Ne激光对聚γ 谷氨酸生产菌地衣芽孢杆菌的诱变作用。     

He—Ne激光血管内照射血液治疗冠心病的临床研究

应用低强度Ｈｅ－Ｎｅ激光血管内照射（ＩＬＩＢ）疗法试治３２例冠心病患者,同时设正常对照２０例,进行血液流变学、血清ＭＤＡ水平及其它相关指标的疗前后对比检测。结果表明所有指标在ＩＬＩＢ治疗后比疗前有显著改善（Ｐ〈０．０１）,与病情好转一致。作者认为ＩＬＩＢ不失为冠心病治疗的有效手段之一,其疗效机理有待进一步研究。     

He—Ne激光照射对离体小鼠巨噬细胞膜电位的影响

低功率Ｈｅ－Ｎｅ激光照射引起细胞膜电位的改变,为激光照射治疗提供理论依据。方法不同能量密度的Ｈｅ－Ｎｅ激光照射离体在噬细胞,用图像分析系统检测Ｃｙａｎｉｎｅ荧光染色的巨噬细胞膜电位的变化。     

不同剂量的He—Ne激光对Raji细胞膜表面SH的影响

本文以离体培养的Ｒａｊｉ细胞为材料,采用ＥＬＬＭＡＮ方法检测了不同剂量的Ｈｅ－Ｎｅ激光对Ｒａｊｉ细胞膜表面ＳＨ含量的影响。发现０．５Ｊ／ｃｍ＾２Ｈｅ－Ｎｅ激光能量可明显增加膜表面ＳＨ含量（Ｐ〈０．０５）。大于或小于此剂量的Ｈｅ－Ｎｅ激光对膜表面ＳＨ含量的影响均不明显（Ｐ〉０．０５）。提示０．５Ｊ／ｃｍ＾２的激光能量对膜有刺激作用。     

YAG与He—Ne激光处理籼稻恢复系干种子的诱变育种效果的研究

用ＹＡＧ,Ｈｅ－Ｎｅ激光处理籼稻处理系恢４８－２干种子,统计了其当代其生物学效应,Ｌ２代的突变频率,几种主要性状的变异系数及广义遗传力,Ｌ２代各处理选１０个突变株与多个不良系配组,表现熟期较早,综合性状较好的组合数,ＹＡＧ激光处理的高于Ｈｅ－Ｎｅ处理的,并选育出了一个较好的新的恢复系－恢４１。     

He—Ne激光照射离体鼠巨噬细胞对线粒体跨膜电势的影响

目的：研究Ｈｅ－Ｎｅ激光照射鼠巨噬细胞对线粒体跨膜电势的影响,及其与激光剂量的关系。方法：用亲脂性阳离子荧光染料Ｒｈｏｄａｍｉｎｅ１２３对鼠巨噬细胞线粒体作荧光标记,以不同的激光剂量照射,采用图像分析系统（ＩＡＳ）和荧光显微镜观察线粒体跨膜电势荧光强度的变化。结果：低功率Ｈｅ－Ｎｅ激光照射５,１０,１５ｍｉｎ,激光剂量分别为０．６４９,１．３８８和２．０８２Ｊ／ｃｍ＾２,巨噬细胞线粒体跨膜电势荧光     

He—Ne激光对天蚕的生理生化效应研究

采用不同剂量的He-Ne激光辐照天蚕卵,当代与对照相比较,孵化率提高、幼虫龄期经过缩短,产生畸变、早熟等个体;对肾血液蛋白质、酯酶同工酶进行PAGE分析,其谱带数和活性也产生了变化,证明He-Ne激光对天蚕不但具有诱变效应,且能获得有价值变异体。     

增强UV—B辐射对蚕豆叶片微粒体膜一些性质的影响

温室条件下,用０,８．６５ｋＪｍ＾－２ｄ＾－１及１１．２ｋＪｍ＾－２ｄ＾－１不同剂量的ＵＶ－Ｂ辐射处理蚕豆幼苗。Ｃａ＾２＋－ＡＴＰａｓｅ及Ｍｇ＾２＋－ＡＴＰａｓｅ的活性在辐射处理期间下降。在处理２１ｄ,Ｔ１和Ｔ２微粒体膜的ＭＤＡ含量明显高于对照,同时ＩＵＦＡ急剧下降,且呈明显的剂量效应。     

环磷酰胺诱发蚕豆体细胞遗传损伤的研究

利用蚕豆根尖研究环磷酰胺的遗传毒性效应, 结果表明:环磷酰胺(0.1~5.0 mg/mL)能够降低蚕豆根尖细胞有丝分裂指数, 使根尖细胞中具有微核、核出芽及核固缩的细胞明显增多, 并诱发染色体结构和行为异常, 产生染色体断片、滞后和桥。环磷酰胺处理组根尖中具有核固缩和微核的细胞数呈剂量依赖性增加, 且与作用时间呈正相关, 而分裂指数的降低也具有剂量和时间效应关系。研究结果表明, 低浓度长时间接触或高浓度短时间接触环磷酰胺均可产生遗传毒害, 因此, 有关的作业人员应注意防护。     

Effects of turgor potentials of epidermal cells neighbouring guard cells on stomatal opening in detached leaf epidermis and intact leaflets of Vicia faba L. (faba bean)

Leaflets of Vicia faba L. (faba bean) were used to determine whether the mechanical forces resulting from the turgor potentials (Φ_p) of the larger epidermal cells neighbouring guard cells play a significant role in regulating stomatal aperture. When Φ_p, of epidermis and Φ_p of bulk leaflet tissue were compared at midday, Φ_p of epidermis were only 15–25% those of bulk leaflet tissue at all but the most negative leaflet water potentials (Φ). When plants were bagged to increase Φ by reducing vapour pressure differences between leaflets and air, Φ_p of bulk leaflet tissue increased to predawn values, but Φ_p, of epidermis increased to only = 20% of predawn values and stomata opened to their widest apertures. Stomatal apertures were positively correlated with Φ_p of bulk leaflet tissue but they were not correlated with Φ_p of epidermis. Reductions in epidermal Φ_p, began predawn, before stomata were open, and reached minimum values at midday, when stomata were open. We conclude that, in Vicia faba, (1) reduction of Φ_p of epidermal cells begins predawn, reducing the counterforce to stomatal opening that would exist if full epidermal turgor were maintained throughout the day, and (2) changes in Φ_p, of leaf epidermal cells do not play a significant role in regulating stomatal aperture.     

Effects of atmospheric CO2 enrichment on early growth of Vivia faba, a plant with large cotyledons

Seedlings of Vicia faba L. were grown in open-top growth chambers at present (P=350μmol^?1) and at elevated (E=700μmol mol^?1) atmospheric CO₂ concentration. The effects of CO₂ enrichment on the first phase of growth after germination were examined over 45 d. There were no positive effects of CO₂ enrichment on growth of the seedlings during this early phase. No differences were observed in leaf area or in total dry weight. No differences were found in morphology or anatomy of the leaves. The numbers of stomatal and epidermal cells, thickness of leaf, of epidermis and of mesophyll cell-layers were unaffected by CO₂ enrichment. Also, no differences were observed in leaf concentrations of chlorophyll, reducing carbohydrates or starch. These results contrast markedly with results from similar experiments on poplar hybrids and Phaseolus vulgaris obtained in the same growth facility. It seems that the intitial growth is under internal control such that the atmospheric CO₂ concentration has no effects. The lack of response in this case may be attributed to the presence and longevity of the large cotyledons which provided available substrate for growth.     

Induction of systemic protection against rust infection in broad bean by saccharin: effects on plant growth and development

Here, we examine the effect of saccharin on the induction of systemic resistance in broad bean (Vicia faba) to the rust fungus Uromyces viciae-fabae. Saccharin was applied to beans at the three-leaf stage, either as a soil drench or by painting the solution on to first leaves. Plants were then challenge inoculated with the rust 1, 6, 10 and 14 d following saccharin treatment, after which they were harvested, assessed for the intensity of rust infection and plant growth measurements conducted. Foliar application of saccharin did not induce systemic protection to rust infection until 14 d after application and was less effective than saccharin applied as a soil drench. When saccharin was applied as a drench, systemic protection was not observed until 6 d after application, but was still apparent in plants 14 d after application of the drench. Irrespective of the method of application, saccharin had no significant effect on fresh and dry weights or leaf area of the plants. Saccharin applied as a drench did, however, reduce the number of leaflets produced.     

Recognition of phlorizin by the carriers of sucrose and hexose in broad bean leaves

Phlorizin (1-[2-(β- d -glucopyranosyloxy)-4, 6-dihydroxyphenyl]-3-(4-hydroxyphenyl)-1-propanone) is a well-known non-transported inhibitor of glucose uptake in animal cells. The effects of this compound were studied on the transmembrane potential difference (PD) of broad bean ( Vicia faba L. cv. Aguadulce) mesophyll cells, and on the uptake of amino acids and sugars by the leaf tissues. Phlorizin (5 m M ) induced a marginal depolarization (7 to 10 mV) of the normal PD (-140 mV), and a slight decrease in the uptake of glycine and serine. By contrast, phlorizin induced a stronger inhibition of the uptake of glucose and 3–O-methylglucose, and more particularly of sucrose uptake and phloem loading. In tissues aged for 12 h, 5 m M phlorizin inhibited the absorption of sucrose from a 1 m M solution by 70%. Kinetic experiments demonstrated that phlorizin acted as a competitive inhibitor for the sucrose carrier and for the hexose carrier. Efflux experiments showed that the counter-exchange of sucrose and of 3–O-methylglucose was also phlorizin-sensitive. Overall, the data show that phlorizin is recognized by the hexose carrier and, more efficiently, by the sucrose carrier of the material investigated, but that it is not transported across the membrane.     

He-Ne激光处理不同时期蚕豆幼苗对抗氧化系统的影响

采用功率为3.50 mW/mm2的He-Ne激光处理不同时期蚕豆,研究其四叶期叶片中丙二醛(MDA)含量,超氧化物歧化酶(SOD)、过氧化物酶(POD)、过氧化氢酶(CAT)活性及同工酶谱的变化。结果表明,与对照相比,He-Ne激光处理不同时期蚕豆,MDA含量均显著降低,且各处理间没有显著差异;SOD、POD、CAT酶活性有不同程度提高。SOD、POD同工酶的酶谱在浸种24小时和胚芽露头期经激光处理后改变,在一叶期处理后没有改变;CAT同工酶谱没有变化;在一叶期处理的三种同工酶谱都没有改变。     

共聚焦显微技术研究SA对蚕豆气孔保卫细胞的影响

水杨酸(salicylic acid,SA)作为植物体内一种内源性的信号分子,具有多种生理功能.实验表明水杨酸以浓度依赖的方式诱导气孔关闭,抑制气孔张开.20U/mL的CAT与SA共同处理时可逆转SA诱导气孔关闭作用的83%~90%.以H2O2荧光探针H2DCFDA结合激光扫描共聚焦显微术直接检测到SA处理可引起保卫细胞内H2O2的产生;在保卫细胞内显微注射CAT可完全阻止SA导致的DCF荧光增强.表明SA诱导的气孔关闭可能与H2O2的产生有关.     

Translocation of labelled assimilates following photosynthesis of 14CO2 by the field bean, Vicia faba

When whole plants were exposed to ¹⁴CO₂, almost the same amount of radioactivity was taken up initially by each leaf regardless of its position on the stem and of the presence of beans at that node. Thus, although developing beans are a powerful sink for assimilated carbon, they do not increase the CO₂ uptake by adjoining leaves.
The distribution of labelled assimilates 6 hours after feeding ¹⁴CO₂ to a single leaf for 1 hour varied with both the position of the treated leaf and the stage of development of the plant. Before any flowers were set most of the radioactivity from all expanded leaves moved downwards to the roots and the stem below the treated leaf (lower stem). Later, during pod-fill, the upper leaves maintained this supply to the roots and lower stem, whilst most of the carbon translocated from the lower and mid-stem leaves went to the beans. However, we found no exclusive relationship between a leaf and the supply to beans developing on the same node.
The amount of radioactivity moving out of a source leaf at a fruiting node increased over successive samplings up to 48 h; the pattern of distribution of the ¹⁴CO₂ however remained virtually unchanged.     

Carrier-mediated uptake of glyphosate in broad bean (Vicia faba) via a phosphate transporter

The possibility that the herbicide glyphosate (N-phosphonomethylglycine) may be taken up in plant cells via a phosphate transporter of the plasma membrane was investigated using protoplasts of broad bean leaves ( Vicia faba L.). Phosphonoformic acid, a powerful inhibitor of phosphate transport in animal cells, was first demonstrated to be a competitive inhibitor of phosphate uptake inbroad bean protoplasts. Glyphosate was able to inhibit phosphate uptake into the protoplasts, and to protect partially the phosphate transporter from inhibition by phosphonoformic acid. Concentration dependence studies showed that glyphosate uptake exhibited a saturable phase at low glyphosate concentrations (0. 5 to 3 μ M ), superimposed by a linear uptake at higher concentrations (up to 100 μ M ). Inhibition of glyphosate uptake by para -chloromercuribenzene sulphonic acid, sodium azide and carbonyl-cyanide- m -chlorophenylhydrazone was much stronger at 1 than at 100 μ M glyphosate. Kinetics indicated that the saturable component of glyphosate transport was competitively inhibited by either phosphate or phosphonoformic acid. It is concluded that glyphosate can be absorbed via a phosphate transporter of the plasma membrane