Molecular modelling of theDolichos biflorus seed lectin and its specific interactions with carbohydrates: α-D-N-acetyl-galactosamine,Forssman disaccharide and blood group A trisaccharide

The three-dimensional structure ofDolichos biflorus seed lectin has been constructed using five legume lectins for which high resolution crystal structures were available. The validity of the resulting model has been thoroughly investigated. Final structure optimization was conducted for the lectin complexed with GalNAc, providing thereby the first three-dimensional structure of lectin/GalNAc complex. The role of theN-acetyl group was clearly evidenced by the occurrence of a strong hydrogen bond between the protein and the carbonyl oxygen of the carbohydrate and by hydrophobic interaction between the methyl group and aromatic amino acids. Since the lectin specificity is maximum for the Forssman disaccharide GalNAc(1–3)GalNAc-O-Me and the blood group A trisaccharide GalNAc(1–3)[Fuc(1–2)]Gal-O-Me, the complexes with these oligosaccharides have been also modelled.     

A comparison of the carbohydrate binding properties of twoDolichos biflorus lectins

The carbohydrate binding properties of theDolichos biflorus seed lectin and DB58, a vegetative tissue lectin from this plant, were compared using two types of solid phase assays. Both lectins bind to hog blood group A + H substance covalently coupled to Sepharose 4B and this binding can be inhibited with free blood group A + H substance. However, the binding of the seed lectin is inhibited byD-GalNAc whereas DB58 binding was not inhbited by any monosaccharide tested, thus suggesting that its carbohydrate combining site may be more extensive than that of the seed lectin. The activities of these two lectins also differ from one another in ability to recognize blood group A + H substance adsorbed on to plastic and in the effects of salt and urea on their carbohydrate binding activities. Neither lectin showed glycosidase activity with p-nitrophenyl -D-GalNAc or p-nitrophenyl -D-GalNAc.     

Nodulation and growth ofLablab purpureus (Dolichos lablab) in relation to rhizobium strain,liming and phosphorus

Summary Greenhouse experiments were done with two purposes: (1) to identify strains of rhizobia effective and acid-tolerant in symbiosis withLablab purpureus, and (2) to determine whether soil acidity or the symbiotic condition increased the phosphate requirement for growth.Five rhizobial strains were tested in one neutral soil, two acid soils, and the two acid soils limed to pH 6.6. In the neutral and limed soils, three of the strains were effective (CB1024, CB756, TAL169), but only two strains (CB756, TAL169) remained effective in acid soil.Strain CB756 and plus-N treatments were further compared in a factorial trial involving combinations of five levels of P with lime, no lime and CaCl₂ treatments, applied to an acid soil. Some of the treatments were also applied to plants inoculated with CB1024. Between the N-fertilized and CB756 treatments there was no clear difference in growth response to applied P, and the critical internal concentration of P for 95% of maximal growth was the same (0.22% shoot dry weight). Increasing P beyond levels needed for maximal growth increased nodulation and N concentration in plants inoculated with CB756. It lowered N concentration in N-fertilized plants. There was evidence suggesting that the P requirement of symbiotic plants increased if the soil was acid, or if CB756 were replaced by CB1024 as microsymbiont; but the critical statistical interactions were not significant.     

Nodulation,nitrogen fixation,leaf area,and sugars content inLablab purpureus as affected by sulfur nutrition

Summary In order to explore interrelations between S nutrition, soluble sugars, leaf area, nodulation and N₂ fixation, greenhouse experiments were done with several levels of S added to perlite-sand cultures or to a moderately S-deficient soil. Sulfur had indirect effects on nodulation and N₂ fixation, possibly by improving sugars supply and N metabolism.In perlite-sand culture, leaf area increased with concentrations of supplied S up to 50 and 200 M for symbiotic and N-treated plants respectively, then decreased at higher concentrations. Plant yield and total sugars content (mg per plant) for the N-treated plants behaved similar to leaf area in response to added S but in the symbiotic plants maximum values were obtained at 100 M S. In soil, Mo had no effect on growth but interacted significantly with S in affecting total sugars content. High levels of S depressed sugars content at low Mo but raised it at high Mo.Sulfur increased the N content of soil-grown plants. It increased the N content of plants grown in perlite-sand culture except at very high levels of S. There was little effect on concentration of N in the shoots. Nitrogen content correlated significantly with leaf area and sugar content, and highly significantly with S concentration in the shoots.     

Structures and kinetics for plant nucleoside triphosphate diphosphohydrolases support a domain motion catalytic mechanism

Extracellular nucleoside triphosphate diphosphohydrolases (NTPDases) are enzymes that hydrolyze extracellular nucleotides to the respective monophosphate nucleotides. In the past 20 years, NTPDases belonging to mammalian, parasitic and prokaryotic domains of life have been discovered, cloned and characterized. We reveal the first structures of NTPDases from the legume plant species Trifolium repens (7WC) and Vigna unguiculata subsp. cylindrica (DbLNP). Four crystal structures of 7WC and DbLNP were determined at resolutions between 1.9 and 2.6 Å. For 7WC, structures were determined for an ‐apo form (1.89 Å) and with the product AMP (2.15 Å) and adenine and phosphate (1.76 Å) bound. For DbLNP, a structure was solved with phosphate and manganese bound (2.60 Å). Thorough kinetic data and analysis is presented. The structure of 7WC and DbLNP reveals that these NTPDases can adopt two conformations depending on the molecule and co‐factor bound in the active site. A central hinge region creates a “butterfly‐like” motion of the domains that reduces the width of the inter‐domain active site cleft upon molecule binding. This phenomenon has been previously described in Rattus norvegicus and Legionella pneumophila NTPDaseI and Toxoplasma gondii NTPDaseIII suggesting a common catalytic mechanism across the domains of life.     

黑皮扁豆凝集素提纯及部分性质研究

采用NaCl抽提、硫酸铵分部沉淀和2步离子交换法从黑皮扁豆中纯化得到一种甘露糖专一凝集素(DPL)。在非变性电泳中纯化的DPL只有一条蛋白带,在还原及非还原条件下的SDS-PAGE中呈现两条蛋白带,其分子量分别为36．8kD和39．8kD;利用FPLC经Sephacryl S-300凝胶过滤测得其表观分子量为155kD,表明DPL由2个α亚基和2个β亚基组成,无二硫键。DPL的等电点为pH6．18,含1．6％糖,为酸性糖蛋白。DPL的热稳定性和pH稳定性,与已报道的甘露糖/葡萄糖专一的豆科凝集素相似。     

扁豆绒毡层发育的超微结构研究

应用透射电镜对扁豆绒毡层发育过程进行了研究,主要结果如下：１）首次发现扁豆绒毡层在发育过程中,经历了二交胞质重组（第一次始于减数分裂末期Ⅱ,第二次始于小孢子发育早期）,使绒毡层细胞的活动呈现３个高峰期（即小孢子母细胞减数分裂期、小孢子四分体期一小孢子早期、小孢子晚期－二胞花粉中期）。２绒毡层细胞的分泌作用有３种形式（渗透分泌、胞吐分泌和自溶）。３．首次观察到绒毡层细胞的内切向壁和径向壁经历了两个周     

Analysis of the amino acid sequences of plant Bowman-Birk inhibitors

Plant seeds contain a large number of protease inhibitors of animal, fungal, and bacterial origin. One of the well-studied families of these inhibitors is the Bowman-Birk family(BBI). The BBIs from dicotyledonous seeds are 8K, double-headed proteins. In contrast, the 8K inhibitors from monocotyledonous seeds are single headed. Monocots also have a 16K, double-headed inhibitor. We have determined the primary structure of a Bowman-Birk inhibitor from a dicot, horsegram, by sequential edman analysis of the intact protein and peptides derived from enzymatic and chemical cleavage. The 76-residue-long inhibitor is very similar to that ofMacrotyloma axillare. An analysis of this inhibitor along with 26 other Bowman-Birk inhibitor domains (MW 8K) available in the SWISSPROT databank revealed that the proteins from monocots and dicots belong to related but distinct families. Inhibitors from monocots show larger variation in sequence. Sequence comparison shows that a crucial disulphide which connects the amino and carboxy termini of the active site loop is lost in monocots. The loss of a reactive site in monocots seems to be correlated to this. However, it appears that this disulphide is not absolutely essential for retention of inhibitory function. Our analysis suggests that gene duplication leading to a 16K inhibitor in monocots has occurred, probably after the divergence of monocots and dicots, and also after the loss of second reactive site in monocots. S. Selvaraj is on leave from Department of Physics, Bharathidasan University, Tiruchirapalli 620 024, Tamilnadu, India Correspondence to: M.R.N. Murthy     

侵染扁豆的三叶草黄脉病毒的鉴定

1987年从泰安表现系统花叶的扁豆上分离到一个分离物B_2,汁液摩擦接种9科38种植物,它可侵染5科10种植物,在扁豆和昆诺藜上引起系统花叶,在苋色藜上引起局部枯斑。该分离物钝化温度为60—65℃,稀释限点为10~(-3)—10~(-4),体外存活期为3—5天。可由桃蚜传播;病毒粒体线条状,大小为700—760×12nm病叶细胞内有风轮状内含体,该分离物与三叶草黄脉病毒的抗血清有明显的-阳性反应。根据这些特性,该病毒属于马铃薯丫病毒组的三叶草黄脉病毒。