A simple diffusion test for soil phosphorus availability

The availability of phosphorus to plants was estimated by a new method based on the diffusion of P from a thin layer of water-saturated stationary soil to a disc of iron oxide coated filter paper. Twenty-one acid Finnish soil samples were tested using four modifications of the method which differed in the duration of the diffusion time and in the thickness of the soil layer. The new diffusion tests were compared with other soil P testing methods and evaluated as indicators of the availability of P to pot-grown barley and oats. Close linear correlations were found between the initial (18 or 42 h) P diffusion rate and the water extractable P contents determined at the extraction ratios of 1:10 and 1:60, respectively (r=0.97–0.99). The amounts of P obtained by the new method were small when the diffusion time was short, but after prolonged diffusion (1 week) the test values were close to the amounts of P taken up by plants. The relationships of plant yield and P uptake with soil P test values were affected by soil acidity. Although the original soil P test values were significantly correlated, the accuracy of all methods drastically improved when the interfering effect of soil acidity was taken into account using a simple pH-correction model. The correlation coefficients (r) between the test values of diffusible P in soil and the uptake of P by plants increased up to 0.97.     

Proteolytic degradation of barley ribulose-1,5-bisphosphate carboxylase/oxygenase and recognition of the fragments by monoclonal antibodies

Limited proteolysis of barley ribulose-1,5-bisphosphate carboxylase/oxygenase (RuBPCO) was effected by treatments with trypsin and Staphylococcus aureus strain V8 protease. Treatment of native RuBPCO with proteases resulted in the degradation of the large subunit (LS) of the enzyme. Trypsin cleaved three fragments from the LS but the S. aureus strain V8 protease cleaved only one. The small subunit (SS) was not affected. In the presence of 0.5 % sodium dodecyl sulfate, RuBPCO degraded into several fragments; some of them were fairly stable. Monoclonal antibodies (Mabs) against barley RuBPCO were applied in immunoblotting analysis to distinguish which of the fragments were recognized. All the Mabs recognized the fragments with molecular masses close to those of the LS. Differences among Mabs were observed in the fragments with low molecular mass. This revised version was published online in June 2006 with corrections to the Cover Date.     

A comparison of several published methods for barley anther culture

A number of methods have been published for barley (Hordeum vulgare L.) anther culture and have gained acceptance in different laboratories. The breeder's requirement is for a compromise method that gives good, repeatable results for a wide range of genotypes. Yet the routine production of spontaneously doubled haploid green regenerants remains difficult. Despite attempts to formulate a widely-applicable anther culture method, the 4 main published methods, compared here with one modified procedure, are quite distinct for a number of important characteristics. The methods interacted strongly with the 3 genotypes, and response ranged from zero to 28 green regenerants per 100 anthers plated. The current methods still require often substantial modification to suit local situations in order that the technology may be exploited by barley breeders.Abbreviations BAP benzylaminopurine - DH doubled haploid - FV final volume - IAA indoleacetic acid - IBA indole-3-butyric acid - MS Murashige & Skoog - PABA para-aminobenzoic acid     

Purification and properties of protein Z – a major albumin of barley endosperm

A major albumin of barley grain, called protein Z, has been purified from endosperm flour. Extraction with 0.05 M β-mercaptoethanol and successive use of (NH ₄)₂SO₄-precipitation, anion exchange at pH 7.5, cation exchange at pH 4.5, and anion exchange at pH 8.0 resulted in a highly pure protein as judged from various electrophoretic and immunoelectrophoretic tests. As protein Z is a major protein component of beer, antibodies towards a protein-rich beer fraction could be used to detect the protein during purification. Protein Z consists of at least four antigenically identical molecular forms with isoelectric points in the range 5.55–5.8, but same molecular mass near 40000. Dimer and, probably, tetramer forms were detected by gel filtration in the absence of reducing agents. Monospecific antibodies towards protein Z were prepared. Immunoelectrophoretic properties of the protein were not affected by treatment at pH 1–13 (30 min at 30°C) or up to 100°C (30 min at pH 7). Commonly grown barley varieties contained about 1.5–2.5 mg protein Z/g grain, but a much lower content (∼ 0.2 mg/g grain) was found in a few varieties. Like barley β-amylase, protein Z was present in both salt-extractable "free" (20–30%) and thiol-extractable "latent" (70–80%) forms in the grain. Protein Z contains 2 cysteine and 20 lysine residues per monomer molecule and is relatively rich in leucine and other hydrophobic residues. Protein Z may contribute up to 5% of the total grain lysine in normal varieties and more than 7% in some high-lysine barleys.     

The effect of kinetin on chlorophyll synthesis in ageing etiolated barley leaves exposed to light

Etiolated barley seedlings lose the ability to produce chlorophyll and soluble protein on exposure to light with increasing age. Similarly, the production of δ-aminolaevulinic acid-dehydratase and succinyl-CoA synthetase is decreased in older etiolated leaves exposed to light. The rate of protochlorophyllide₆₅₂ regeneration decreased well before the rates of exogenous δ-aminolaevulinic acid conversion to protochlorophyllide₆₃₂ was affected by ageing. Application of kinetin retarded these ageing symptoms in the etiolated leaves.     

ABA-induced proline accumulation in barley leaf segments: Dependence on protein synthesis

The kinetics of proline accumulation in barley ( Hordeum vulgare L. cv. Georgie) leaf segments showed a lag phase of ca 3 h when the increase was induced by abscisic acid (ABA), but not when the accumulation of the imino acid was promoted by isobutyric acid (IBA). Cycloheximide (CHI) supplied together with ABA, either from the beginning of the treatment or some time before the end of the lag phase, completely abolished ABA-induced proline accumulation, whereas no block was observed when the inhibitor was supplied after the lag phase. Cordycepin (COR) exibited a similar effect. The IBA-induced increase in proline was not influenced by CHI for at least 5 h.
When segments were pretreated with ABA for a period longer than the lag phase in the absence of salts in the external medium, there was no significant increase in proline. If KCI was added to the incubation medium after such a pretreatment, however, proline increased even after removal of the hormone from the external medium. This increase in proline occurred without any lag phase, and was only partially inbibited by CHI and rapidly and totally blocked by fusicoccin (FC). These results suggest that some protein, characterized by a fast turnover and possibly conferring the sensitivity to KCI, is synthesized during the early hours (lag phase) of the ABA treatment.
The synthesis of this protein(s) does not seem to be involved in the increase in proline induced by IBA and is thus a peculiar aspect of that mediated by ABA.     

粉葛PtCHI基因的克隆、原核表达和亚细胞定位

为探究葛根品种间异黄酮类物质代谢关键酶基因PtCHI的分子机制差异，并揭示其品种间异黄酮物质含量差异的原因，该研究以野葛品种‘桂葛8号’和粉葛品种‘桂葛1号’为材料，经乙醇提取并通过高效液相色谱仪对野葛和粉葛中葛根素和总黄酮的含量进行测定，基于已报道的野葛CHI基因，通过同源克隆方法分离粉葛中PtCHI基因，并在体外进行蛋白表达，同时在拟南芥原生质体中研究PtCHI基因的定位。结果表明：(1)野葛中的葛根素含量显著高于粉葛的，野葛的总黄酮含量也高于粉葛但未达到显著水平。(2)成功分离到粉葛PtCHI基因，长度为742 bp且包含672 bp完整的ORF框，编码223个氨基酸，与野葛的CHI基因具有99%的同源性。(3)CHI基因在粉葛中的表达量为茎>根>叶子，在野葛中则为根>茎>叶子，除叶子外野葛中CHI基因的表达量均显著高于粉葛。(4)经预测，粉葛PtCHI蛋白为稳定的亲水性蛋白且大小为27.8 kD,二、三级结构以α-螺旋为主，具有25个磷酸化位点，与野葛、大豆和乌拉尔甘草的亲缘关系较近，与F3H2、F3H、4CL4、DFR2及CHS发生互作的可能性较大。(...     

Isolation,structure elucidation and in-vitro evaluation of new trisubstituted Tetrahydrofuran Lignans from Rabdosia lophanthoides var. gerardiana as anti-inflammatory agents

Four new trisubstituted tetrahydrofuran lignans, named (−)-sesaminone-rutinoside (1), (+)-episesaminone-rutinoside (2) and rabdosiacosides B (3) and C (4) were isolated from the air-dried whole herbs of Rabdosia lophanthoides var. gerardiana together with two known compounds, (+)− 1-hydroxypinoresinol-1-β-d-glucoside (5) and rosmarinic acid (6). The structures of these new lignans were elucidated by a combination of mass spectrometry, 1D and 2D NMR experiments including distortionless enhancement by polarization transfer, ¹H–¹H correlation, heteronuclear single quantum coherence, heteronuclear multiple bond correlation, and nuclear Overhauser effect spectroscopies. Both the cell viability and their anti-inflammatory effects of the lignans were further studied. Among them, no significant cytotoxic activity was exhibited. Compound 4 dramatically suppressed LPS-induced nitric oxide release and reduced the release of the pro-inflammatory cytokines TNF-α and IL-6 in a dose-dependent manner. Overall, our findings indicate that compound 4 was noteworthy in reducing LPS-induced inflammatory responses in RAW264.7 macrophages.     

Regulation of germination by targeted mutagenesis of grain dormancy genes in barley

High humidity during harvest season often causes pre-harvest sprouting in barley (Hordeum vulgare). Prolonged grain dormancy prevents pre-harvest sprouting; however, extended dormancy can interfere with malt production and uniform germination upon sowing. In this study, we used Cas9-induced targeted mutagenesis to create single and double mutants in QTL FOR SEED DORMANCY 1 (Qsd1) and Qsd2 in the same genetic background. We performed germination assays in independent qsd1 and qsd2 single mutants, as well as in two double mutants, which revealed a strong repression of germination in the mutants. These results demonstrated that normal early grain germination requires both Qsd1 and Qsd2 function. However, germination of qsd1 was promoted by treatment with 3% hydrogen peroxide, supporting the notion that the mutants exhibit delayed germination. Likewise, exposure to cold temperatures largely alleviated the block of germination in the single and double mutants. Notably, qsd1 mutants partially suppress the long dormancy phenotype of qsd2, while qsd2 mutant grains failed to germinate in the light, but not in the dark. Consistent with the delay in germination, abscisic acid accumulated in all mutants relative to the wild type, but abscisic acid levels cannot maintain long-term dormancy and only delay germination. Elucidation of mutant allele interactions, such as those shown in this study, are important for fine-tuning traits that will lead to the design of grain dormancy through combinations of mutant alleles. Thus, these mutants will provide the necessary germplasm to study grain dormancy and germination in barley.