Influence of cocksfoot streak virus on the growth of single cocksfoot plants

Healthy and streak-virus-infected cocksfoot plants of a single genotype were examined over a 2-year period. In the first year infection decreased tillering by about 40%, but in pot-grown plants individual tiller weights were 30% higher so dry-matter yield was decreased by only 10%. In the second year the larger tiller weights compensated completely for decreased tillering. No similar compensation was observed in field-grown plants. The virus had the largest effects when soil fertility was highest, healthy plants producing significantly greater responses to nitrogen effects, but potassium, at certain times of the year, produced larger tiller weights in infected than in healthy plants. Infection decreased dry-matter yield more in frequently than in infrequently cut plants. Infection greatly decreased the number of vegetative but not of fertile tillers. Infected plants tended to flower earlier and produced fewer, slightly smaller, viable seeds.     

A Method for in Vitro Storage of Lolium multiflorum Lam

A means of storing Lolium multiflorum Lam. stock plants in vitrohas been developed over a period of three years. Variousexplantsand cultureconditions were examined. Shoot tips 0.3–0.9mm long were found to be best for establishing storage culturesbecause they gave a high yield of plantlets in culture and importantpathogens are eliminated. For sub-culturing, after each annualcycle of storage at 2–4 °C, shoot tips, tiller buds,tiller bases and nodes can be used. Tiller buds were most abundantand best for increasing the number of stored plantlets whennecessary. There was no advantage of including an auxin in theculture medium for shoot tips and Murashige and Skoog's mediumwith 0.2 mg l^–1 kinetin has been adopted for initiating,sub-culturing and storing cultures. The optimum temperaturerange for regenerating plantlets was 20–25 °C. Lightwas necessary for a high rate of plantlet regeneration and lightquality and intensity affected their growth. Lolium multiflorum Lam., ryegrass, storage in vitro, tissue culture     

Association of cocksfoot mild mosaic and cocksfoot streak viruses in Dactylis glomerata and their simultaneous transmission by aphids

Macrosiphum (Sitobion) fragariae transmitted cocksfoot mild mosaic and cocksfoot streak viruses two to three times more frequently from plants in which they occurred together than from plants in which they occurred alone. In cells of doubly infected plants, particles of the two viruses commonly occurred in close association.     

Some properties of cocksfoot mottle virus

Cocksfoot mottle virus (CFMV) was transmitted by manual inoculation of sap to cocksfoot (Dactylis glomerata L.), wheat, oats and barley, but not to nineteen other monocotyledonous and thirteen dicotyledonous plant species. The virus was also transmitted by cereal leaf beetles (Lema melanopa L.). Adult beetles infected plants more frequently than larvae, and remained infective for up to 2 weeks after they had fed on infected plants. Seed from infected cocksfoot and oat plants produced virus-free seedlings. The infectivity of sap was lost during 10 min. at 65° C., and 2 weeks at 20° C., but survived many months at — 15° C. Purified virus preparations, made by various methods, contained numerous nearly spherical particles, about 30 mμ in diameter. In electron micrographs some of the particles were penetrated by negative stain though most appeared intact. However, all the particles migrated together in a centrifugal (sedimentation coefficient = 118 S) or electrophoretic field. The ultraviolet absorption spectrum, and the phosphorus and nitrogen contents of the virus preparations, were typical of a nucleoprotein containing about 25 % nucleic acid. Serological tests failed to show any relationship between CFMV and eleven other viruses with particles of similar shape and size.     

Epidemiology of cocksfoot mottle virus

Cocksfoot mottle virus (CFMV) was found to be widespread in cocksfoot seed crops in the East Midlands in the third harvest year and once present in the crop spread rapidly. Pot experiments with single cocksfoot plants showed that autumn infection with CFMV resulted in a significant reduction in the number of flowering tillers and weight and size of seed produced the following year. The spread of CFMV in experimental cocksfoot leys was studied; leys cut for conservation showed more infection than leys grazed by sheep, and increasing nitrogen application resulted in higher disease incidence. The disease increased rapidly in conserved leys in 1967 and its spread was associated with cutting by a forage harvester after the virus had been introduced into the crop in the autumn, possibly by the vector Lema melanopa. Animal grazing and cutting implements seemed to be more important agencies in disease spread than the vector.     

Properties of cocksfoot streak and cocksfoot cryptic, two viruses infecting cocksfoot (Dactylis glomerata) in Scotland

A Scottish isolate of cocksfoot streak virus (CSV-S) was found to have flexuous filamentous particles which, in sap of infected cocksfoot plants, had a modal length of 712 nm. It was transmitted from infected to healthy cocksfoot plants in a non-persistent manner by Myzus persicae and by mechanical inoculation of infective sap extracts containing an anti-oxidant. Apart from cocksfoot, mechanical inoculation of infective sap succeeded in infecting only four of 22 plant species tested. The infectivity of sap extracts containing 0.2% thioglycerol was lost after heating for 10 min at 55^oC but not 50^oC, storage at room temperature for 48 but not 24 hours, and after diluting 10^-2to 10^-3. Highly purified preparations of CSV-S particles sedimented as a single component with a sedimentation coefficient of 139S and had a buoyant density in rubidium bromide of 1.31 g/cm³. Virus particles were composed of one protein and one ssRNA species with estimated M_r of 31 000 and 3.2 times 10⁶respectively. In ELISA, an antiserum prepared to CSV-S detected the virus in all aerial parts of infected cocksfoot plants and, when present in the ratio of 1 infected leaf: 1000 healthy leaves. Both CSV-S-infected and -uninfected cocksfoot also contained a previously undescribed virus with isometric particles c. 30 nm in diameter. This virus, named cocksfoot cryptic virus (CCV), was seed-borne in two cvs of cocksfoot tested and its particles contained two dsRNA species of estimated M_r of 1.14 times 10⁶and 1.27 times 10⁶. Despite the fact that particles of CSV-S were largely free from CCV particles following exclusion chromatography on agarose beads prior to immunisation, immunoelectron microscopy (IEM) showed that the antiserum prepared to CSV-S also contained some antibodies to CCV. Evidence from IEM suggested a possible distant serological relationship of CCV to ryegrass and beet (BCV 1 or BCV 2, or both) cryptoviruses, all members of sub-group A of crypto viruses.     

Properties of cocksfoot streak and cocksfoot cryptic, two viruses infecting cocksfoot (Dactylis glomerate) in Scotland

A Scottish isolate of cocksfoot streak virus (CSV-S) was found to have flexuous filamentous particles which, in sap of infected cocksfoot plants, had a modal length of 712 nm. It was transmitted from infected to healthy cocksfoot plants in a non-persistent manner by Myzus persicae and by mechanical inoculation of infective sap extracts containing an anti-oxidant. Apart from cocksfoot, mechanical inoculation of infective sap succeeded in infecting only four of 22 plant species tested. The infectivity of sap extracts containing 0.2% thioglycerol was lost after heating for 10 min at 55^oC but not 50^oC, storage at room temperature for 48 but not 24 hours, and after diluting 10-2 to 10-3. Highly purified preparations of CSV-S particles sedimented as a single component with a sedimentation coefficient of 139S and had a buoyant density in rubidium bromide of 1.31 g/cm3. Virus particles were composed of one protein and one ssRNA species with estimated Mr of 31 000 and 3.2 times 106 respectively. In ELISA, an antiserum prepared to CSV-S detected the virus in all aerial parts of infected cocksfoot plants and, when present in the ratio of 1 infected leaf: 1000 healthy leaves. Both CSV-S-infected and -uninfected cocksfoot also contained a previously undescribed virus with isometric particles c. 30 nm in diameter. This virus, named cocksfoot cryptic virus (CCV), was seed-borne in two cvs of cocksfoot tested and its particles contained two dsRNA species of estimated Mt of 1.14 times 106 and 1.27 times 106. Despite the fact that particles of CSV-S were largely free from CCV particles following exclusion chromatography on agarose beads prior to immunisation, immunoelectron microscopy (IEM) showed that the antiserum prepared to CSV-S also contained some antibodies to CCV. Evidence from IEM suggested a possible distant serological relationship of CCV to ryegrass and beet (BCV 1 or BCV 2, or both) cryptoviruses, all members of sub-group A of cryptoviruses.     

Micropropagation of Rosmarinus officinalis L.

Single-node stem segments of Rosmarinus officinalis L. var. genuina forma erectus proved better explants than shoot tips (ca. 2 cm long) for extablishment of field-grown plants in aseptic cultures. Benzylaminopurine was far more effective than kinetin for shoot induction in shoot tips excised from aseptically-grown plants. Maximum numbers of shoot buds (ca. 14) were formed per explant at 0.2 mgl^-1 benzylaminopurine in 30 days. After further growth of isolated shoots and treatment with 0.25 mgl^-1 indolepropionic acid for 7 days, 80% shoots produced roots. In vitro raised plantlets were successfully grown in soil to plants. About 5,000 plants could be produced from a single nodal segment in 1 year.NBRI Research Publication No. 195 (N.S.)     

Influence of cocksfoot streak virus on the growth of cocksfoot swards

Small experimental swards of three types-healthy, 50% and 100% streak-virus-infected-were established from single tillers of randomly selected cocksfoot genotypes. In these swards 44% of infected plants died within 2 years compared with 21% of healthy plants. Mortality of infected plants was not increased by the presence of healthy plants in the same sward. In swards containing both healthy and infected plants, increased growth of healthy plants compensated for the low yield of infected ones only when the swards were frequently defoliated. Infrequent cutting apparently allowed infected plants to check the growth of healthy ones, and 50% infected swards yielded little more than 100% infected swards. This difference in response was attributed to differences in the growth habits of healthy and infected plants. Few initially healthy plants became infected during 2 years of the experiment.     

Electron microscopy of cocksfoot streak virus and its differentiation from ryegrass mosaic virus in naturally infected Dactylis glomerata plants

The length and rigidity of some cocksfoot streak virus (CSV) particles were greater (1) in ammonium molybdate negative stain at pH 5 than at pH 8 and (2) when magnesium was added either directly to extracted plant sap or indirectly via increased plant uptake. Most CSV particles were flexuous and 750–760 run long in low concentrations of magnesium but many were rigid and 800–810 nm long in higher concentrations. In sodium phosphotungstate and ammonium molybdate at pH 5, frequency distributions of particle lengths from cocksfoot plants infected with both CSV and ryegrass mosaic virus (RMV) produced two modal peaks, one at less than 700 nm (RMV) and the other at more than 750 nm (CSV); in ammonium molybdate at pH 8, however, only one peak (at 725 nm) was resolved. In ultrathin sections of CSV-infected cocksfoot leaves, virus-like particles were scattered or in bundles within the cytoplasm, or aligned in aggregates near the tonoplast. Some cells contained pinwheel inclusions, often with attached or associated laminar plates and occasionally with scroll-like or circular tubes. These CSV-induced inclusions were easily distinguished from those induced by RMV, even when both types occurred in the same cell.     

Shoot tip culture and cryopreservation for eradication of Apple stem pitting virus (ASPV) and Apple stem grooving virus (ASGV) from apple rootstocks ‘M9’ and ‘M26’

This study attempted to eradicate Apple stem pitting virus (ASPV) and Apple stem grooving virus (ASGV) from virus‐infected in vitro shoots of apple rootstocks ‘M9’ and ‘M26’ using shoot tip culture and cryopreservation. In shoot tip culture, shoot tips (0.2 mm in length) containing two leaf primordia failed to show shoot regrowth. Although shoot regrowth rate was the highest in the largest shoot tips (1.0 mm in length) containing four leaf primordia, none of the regenerated shoots was virus‐free. Shoot tips (0.5 mm in length) containing two and three leaf primordia produced 100% and 10% of ASPV‐free shoots, respectively, while those (1.0 mm) containing four leaf primordia were not able to eradicate ASPV. ASGV could not be eradicated by shoot tip culture, regardless of the size of the shoot tips tested. In cryopreservation, shoot tips (0.5 mm in length) containing two leaf primordia did not resume shoot growth. Although 1.0‐mm and 1.5‐mm shoot tips gave similarly high ASPV‐free frequencies, the latter had much higher shoot regrowth rate than the former. Very similar results of shoot regrowth and virus eradication by shoot tip culture and cryopreservation were observed in both ‘M9’ and ‘M26’. Histological observations showed that only cells in upper part of apical dome and in leaf primordia 1–3 survived, while other cells were damaged or killed, in shoot tips following cryopreservation. Virus immunolocalization found ASPV was not detected in upper part of apical dome and leaf primordia 1 and 2, but was present in lower part of apical dome, and in leaf primordium 4 and more developed tissues in all samples tested. ASPV was also detected in leaf primordium 3 in about 16.7% and 13.3% samples tested in ‘M9’ and ‘M26’. ASGV was observed in apical dome and leaf primordia 1–6, leaving only a few top layers of cells in apical dome free of the virus. Different abilities of ASPV and ASGV to invade leaf petioles and shoot tips were also noted.     

Cytopathology of Shoot Apical Meristem of Hop Plants Infected with Hop Stunt Viroid11)

Shoot apical meristems of hop plants infected with hop stunt viroid (HSV) were examined for cytopathic changes. No measurable changes in ultrastructure were found in shoot tip 0.2 mm long bearing apical dome and two pairs of the primordia, whereas in the 3rd leaf primordium cell walls were undulate and/or frequently were irregular in thickness. These cell wall abnormalities were not observed in comparable shoot tips of the uninoculated hop plants or HSV-free hop plants obtained by meristem tip culture.     

Cryopreservation of chestnut by vitrification of <Emphasis Type="Italic">in vitro</Emphasis>-grown shoot tips

Summary Plants of European chestnut (Castanea sativa) have been consistently recovered from cryopreserved in vitro-grown shoot apices by using the vitrification procedure. Factors found to influence the success of cryopreservation include the source of the shoot tips (terminal buds or axillary buds), their size, the duration of exposure to the cryoprotectant solution, and the composition of the post-cryostorage recovery medium. The most efficient protocol for shoot regrowth employed 0.5–1.0 mm shoot tips isolated from 1 cm-long terminal buds that had been excised from 3–5-wk shoot cultures and cold hardened at 4°C for 2 wk. The isolated shoot tips were precultured for 2d at 4°C on solidified Gresshoff and Doy medium (GD) supplemented with 0.2M sucrose, and were then treated for 20 min at room temperature with a loading solution (2M glycerol+0.4M sucrose) and for 120 min at 0°C with a modified PVS2 solution before rapid immersion in liquid nitrogen (LN). After 1 d in LN, rapid rewarming and unloading in 1.2M sucrose solution for 20 min, the shoot tips were plated on recovery medium consisting of GD supplemented with 2.2 μM benzyladenine, 2.9 μM 3-indoleacetic acid, and 0.9 μM zeatin. This protocol achieved 38–54% shoot recovery rates among five chestnut clones (three of juvenile origin and two of mature origin), and in all cases plant regeneration was also obtained.     

Ecotype differentiation and coexistence of two parapatric tetraploid subspecies of cocksfoot (Dactylis glomerata) in the Alps

Two tetraploid subspecies of Dactylis glomerata L., subsp. reichenbachii (Hausm.) Stebbins et Zohary and subsp. glomerata , occur in the French Alps. The former is confined to dolomitic, south-facing, alpine lawns above 2000 m, whereas the latter occurs in non-dolomitic habitats in subalpine meadows mainly below 1900 m. Previous studies of allozyme variation have shown that genetic introgression between the two subspecies occurs over large areas. By contrast, morphologically intermediate individuals only occur in an extremely narrow area, suggesting that the morphological and physiological differences between the two subspecies is of adaptive significance. A reciprocal clone transplant experiment was set up to examine (1) any genetic differences between subspecies indicative of ecotypic differentiation in relation to habitat characteristics and (2) the level of phenotypic plasticity in the two subspecies. Genetic differentiation was confirmed by a statistically significant taxon × site interaction effect in anova for all traits studied. The glomerata populations produced more tillers, longer leaves and higher culms in all sites, especially in their home environment. However, reichenbachii populations produced more seeds than the glomerata populations in the original reichenbachii environment, suggesting ecotypic differentiation between the two subspecies. This result might also explain why the glomerata subspecies is unable to colonize dolomitic habitats occupied by the reichenbachii subspecies. The reichenbachii populations showed less plasticity than the glomerata populations for leaf length and floriferous tiller number, a result which is discussed in the context of the response of plants from productive and non-productive habitats to environmental variation.     

Properties of Scottish isolates of cocksfoot mild mosaic virus and their comparison with others

Two isolates of cocksfoot mild mosaic virus obtained from cocksfoot (Dactylis glomerata) in Scotland differed in symptomatology, and apparently in host range, from isolates obtained in Germany and Wales. They were serologically more closely related to a Dutch isolate from cocksfoot, and to a Scottish isolate from timothy (Phleum pratense), than was the German isolate from cocksfoot. The Scottish isolate from timothy was somewhat more virulent than, but serologically closely related to a Welsh isolate from timothy. Particles of Scottish isolates from cocksfoot and timothy were best preserved for electron microscopy by fixation with osmium tetroxide. In 1.0 m KCl or 0.01 m ethylene diamine tetraacetate they were stable at pH 5.2–5.3 but unstable above pH 7; they were disrupted by 0.5% sodium dodecyl sulphate. The particles contained major and minor RNA components of mol. wt c. 1.5. 10⁶(RNA-1) and 0.5. 10⁶(RNA-2) respectively, together with polydisperse RNA of intermediate mol. wt and protein of mol. wt c. 27 000. In CsCl gradients, major and minor nucleoprotein components of density 1.39 and 1.38 g/ml respectively were distinguished. The less dense particles contained a larger proportion of intermediate-sized RNA molecules and of RNA- 2 , and a smaller proportion of RNA- 1 , than did the denser particles. Particles seem to contain either RNA-1 or various combinations of smaller RNA molecules. Despite the differences in antigenic constitution, symptomatology and particle stability between virus isolates obtained from cocksfoot and timothy in different countries, these isolates seem sufficiently similar to be considered one virus.     

Photosynthesis of natural cocksfoot populations under water and salt stresses

Sampling of natural cocksfoot (Dactylis glomerata L.) populations was carried out on the O Morrazo peninsula in NW Spain, characterized by a strong moisture gradient. The plants were kept in greenhouse under standard conditions. Nevertheless, they differ in height of plants, length and width of flag leaves, panicle size, stomatal density and size as well as in flowering period. The effects of two levels of soil water deficit and two levels of salinity on photosynthetic rate were tested. One population was exceptionally well adapted to its original environment with great tolerance to water deficit and salinity     

植物茎分枝的分子调控

植物茎分枝结构决定了不同植物的不同形态结构.本文从腋生分生组织的发生、腋芽的生长两个方面综述了近年来植物分枝发生发育相关的分子机理研究及其进展.发现在不同植物中腋分生组织形成的基本机制是相似的,LS（lateral suppressor）及其同源基因在不同植物中都参与腋生分生组织的形成,而BL(blind)及其同源基因也参与调控腋生分生组织的形成.腋生分生组织的形成可能也是受激素调控的.目前,对腋芽生长的分子调控机制的认识主要集中于生长素通过二级信使的作用调控腋芽的生长.而生长素调控腋芽生长的机制已经较为清楚的有两条途径：一是生长素通过抑制细胞分裂素合成来调控腋芽的生长;另一途径是一种类胡萝卜素衍生的信号物质参与生长素的运输调控(MAX途径)来调控腋芽的生长.最新研究表明,TB1的拟南芥同源基因在MAX途径的下游负调控腋芽的生长.此外,增强表达OsNAC2也促进腋芽的生长.     

In vitro Micrografting of Mature Pistachio (Pistacia vera var. Siirt)

The success of various in vitro micrografting methods of shoot tips of pistachio (Pistacia vera L. var. Siirt) have been examined. Excised zygotic embryos that germinated in vitro were used as rootstocks. Current year shoot tips from mature trees of pistachio micrografted onto in vitro juvenile rootstocks, resulted in the restoration of shoot-bud proliferation. Variables tested include a size of microscion, grafting method, effects of culture medium and effects of time of the year at which shoot tips were used. The results indicate that the easiest and most successful method for grafting was slit micrografting. High levels of micrograft take were achieved with 2–4 mm (56.75%) and 4–6 mm (79.25%) long scions obtained from the regenerated shoot tips. The survival rate of the shoot tips was directly related to time of the year. The best growth of microscion was obtained with the in vitro forced shoot tips rather than with shoot tips excised from tree. Slow growth and lack of axillary shoot development on the micrografts was noticeable when the micrografts were cultured on hormone-free and germination medium. In vitro micrografted plantlets were successfully weaned and no problems were encountered with the establishment of micrografted plants in vivo.     

Accelerated Early Growth of Rice at Elevated CO2 (Is It Related to Developmental Changes in the Shoot Apex?)

The influence of elevated CO2 on the development of the shoot apex and on subsequent vegetative growth and grain yield was investigated using rice (Oryza sativa L. cv Jarrah) grown in flooded soil at either 350 or 700 [mu]L CO2 L-1. At 8 d after planting (DAP), elevated CO2 increased the height and diameter of the apical dome and lengths of leaf primordia and tiller buds but had no effect on their numbers. By 16 DAP, there were five tiller buds in the apex at 700 [mu]L CO2 L-1 compared with only three tiller buds at 350 [mu]L CO2 L-1. These changes in development of the shoot apex at high CO2 were forerunners to faster development of the vegetative shoot at elevated CO2 between 11 and 26 DAP as evidenced by increases in the relative growth rates of the shoot and tillers. Accelerated development at high CO2 was responsible for the 42% increase in tiller number at the maximum tillering stage and the 57% enhancement of grain yield at the final harvest. The link between high CO2 effects on development during the first 15 DAP and final tiller number and grain yield was demonstrated by delaying exposure of plants to high CO2 for 15 d. The delay totally inhibited the tillering response to high CO2, and the increase in grain yield of 20% arose from a greater number of grains per panicle. Consequently, it can be concluded that accelerated development in the shoot apex early in development is crucial for obtaining maximum increases in grain yield at elevated atmospheric CO2 concentrations.