The distribution of poplar mosaic virus in hybrid poplars and virus detection by ELISA

Purified poplar mosaic virus (PMV) at a concentration of 8 ng/ml was readily detected by enzyme-linked immunosorbent assay (ELISA). Bioassay in Nicotiana megalosiphon was more sensitive (detecting 1–4 ng/ml) and latex flocculation less sensitive (c. 25 ng/ml) than ELISA assays. While the foliar sap of fresh, naturally-infected poplars (e.g. Populus. euramericana cv. Robusta) was not infective at dilutions greater than 2 . 10–², ELISA easily detected PMV antigen when sap was diluted 4 . 10–³ in buffer or when one part of infected tissue was triturated with 99 parts healthy leaf. Furthermore, although sap from poplar leaves stored at -20 °C for 6 months was not infective, PMV was still detectable in ELISA tests. PMV antigen in poplar leaves was not all pelleted after centrifugation for 2.5 h at 130 000 g yet parallel tests using unbuffered sap from systemically infected Nicotiana megalosiphon foliage showed that infectivity was restricted to the pellet. In poplar foliage, the concentration of PMV antigen was generally greatest where symptoms were most obvious; least antigen was detected in the overwintering leaves located at the bases of long shoots. In winter, when root and inner bark tissue in the trunk was an erratic source of PMV, the virus was readily detected in buds, the concentration being greatest in the bases, including the meristem, of terminal buds. Propagation from single node cuttings of P. euramericana cv. Regenerata allowed the selection of clones that consistently showed either ‘severe’ or ‘mild’ foliar symptoms. The associated virus isolates also infected another poplar clone causing symptoms characteristic of their source. ELISA consistently detected less PMV antigen in field-grown cv. Regenerata than in cv. Robusta foliage, but this was reversed when the associated virus isolates were propagated in Nicotiana glutinosa at 24 °C. During 6 yr, 21 out of 127 poplars at a site in Western England, became infected with PMV. By contrast, in Eastern England, none of 46 were infected. The aphids Pterocomma populea and Myzus persicae did not transmit PMV.     

Phylogenetics of gall-inducing thrips on Australian Acacia

Analysis of DNA sequence data from four genes ( Elongation Factor-1 α, wingless , 16S rDNA and cytochrome oxidase I ) yielded a well-resolved, well-supported phylogeny for all 21 species of gall-inducing thrips found on Australian Acacia. This phylogeny was then used to investigate the evolution of various behavioural and life history traits, and to examine the level of agreement with the taxonomy of the group. Our results suggest that there may have been a single origin of soldier castes in gall-inducing thrips. Examination of the distribution of the three primary life history strategies employed by these thrips (pupating in the gall, pupating in soil with soldier castes and pupating in soil without soldier castes) indicates that two of the strategies may have evolved as a result of factors associated with host plant affiliations or through parasite pressure. Our phylogeny does not support the existing generic classification of the group in that the genera are not monophyletic, nor does it lend itself to a clear solution to improve the classification in accordance with the phylogeny.     

Tropical acid streams – the chironomid (Diptera) response in northern Australia

1. Chironomidae, sampled by interception of drifting cast pupal exuviae, responded to inputs of acid, heavy metal-rich waters in a seasonally flowing tropical stream in northern Australia.
2. Responses included gain of distinctive (indicative) taxa, loss of some species typical of pristine conditions, and increase in species richness.
3. Experimental manipulation (upstream diversion) of a mine adit entry showed that these responses were the result of change in water quality.
4. The higher species richness at low pH, which is contrary to temperate studies, may be explained by the large tropical (Australian and south-east Asian) pool of species tolerant of naturally occurring acidic aquatic habitats.
5. The structure and responses of the exuvial-assessed chironomid community matched long-term larval data.     

Initiation of Cellulose Biosynthesis

IN spite of much investigation the problem of the molecular mechanism of cellulose synthesis remains unsolved¹. Hexose phosphates², sugar nucleotides^3–6 and a glycolipid^7–9 have been suggested as the precursor of cellulose. Implicit in all these investigations is the supposition that a single substrate suffices for the synthesis. We describe here some preliminary observations which seem to throw new light on the possible mechanism.     

Changes in the Free Amino Compounds in Young Tomato Plants in Light and Darkness with particular Reference to {gamma}-Aminobutyric Acid

Tomato plants were grown to the five-leaf stage under uniformconditions in a growth room with a daily light period of 15h. Plants were sampled at intervals through 24 h periods andthe free ninhydrin-positive compounds determined in roots, bleedingsap, stems and shoots (mainly leaves), using ion-exchange columnchromatography and a lithium-buffer separation system. The compoundspresent and their range of concentrations are given for twooccasions: after illumination for 8 hand after 5 h of darkness. Data for -aminobutyric acid (GAB), glutamic acid, glutamine,alanine, aspartic acid and ammonia are summarized graphicallyfor all occasions and for all parts of the plant; asparaginefor sap only. The data were examined for correlations betweenthese substances for both light and dark conditions. Relative amounts of free acids were: root glutamine> glutamicand GAB > aspartic > alanine; bleeding sap glutamine >asparagine > GAB > aspartic> alanine; stem glutamine> glutamic > GAB and aspartic > alanine; shoot (leaf)GAB and glutamine > aspartic > alanine and glutamic. Patternsof change were as follows: in the root GAB and glutamic weresimilar and unlike glutamine; alanine did not change;sap ammonia,GAB and alanine were parallel, glutamine was similar to theseonly in light; in the stem glutamine and glutamic tended toaccumulate in parallel in light, but GAB did not; in the shoot(leaf) GAB and glutamine were similar except that the formeraccumulated more rapidly in the initial light period; glutamicacid and alanine were similar to each other but distinct fromGAB and glutamine. The relatively large amounts of GAB in tomato plants and themagnitude of the changes occurring in light and darkness seemindicative of its importance as a temporary storage productfor protein amino acids, but the factors controlling accumulationand utilization in different parts of the plant are unknown.