Isolation and characterization of an ipt gene from the Ti plasmid Bo542

Summary A 1.9 kb clone of the T-DNA region of the Agrobacterium tumefaciens Ti plasmid Bo542 which exhibited homology to the isopentenyl transferase (ipt) locus of pTiA6 was identified by low stringency DNA hybridization. Introduction of this segment of pTiBo542 DNA into cells of Nicotiana tabacum or N. glauca caused tumor formation in vivo, and allowed hormone independent growth in vitro. Furthermore, this DNA segment complemented ipt mutant strains of A. tumefaciens, restoring their ability to cause tumors on Kalanchöe leaves and tomato stems. The complete DNA sequence of this segment has been determined, revealing an open reading frame homologous to other known Agrobacterium ipt genes.     

Draft genome sequence of Novosphingobium nitrogenifigens Y88(T)

Novosphingobium nitrogenifigens was originally isolated from pulp and paper mill wastewater, a low-nitrogen, high-carbon environment. N. nitrogenifigens is the first known nitrogen-fixing, polyhydroxyalkanoate-accumulating sphingomonad, and we report the annotated draft genome sequence of the type strain Y88(T) here.     

Golgi Enrichment and Proteomic Analysis of Developing Pinus radiata Xylem by Free-Flow Electrophoresis

Our understanding of the contribution of Golgi proteins to cell wall and wood formation in any woody plant species is limited. Currently, little Golgi proteomics data exists for wood-forming tissues. In this study, we attempted to address this issue by generating and analyzing Golgi-enriched membrane preparations from developing xylem of compression wood from the conifer Pinus radiata. Developing xylem samples from 3-year-old pine trees were harvested for this purpose at a time of active growth and subjected to a combination of density centrifugation followed by free flow electrophoresis, a surface charge separation technique used in the enrichment of Golgi membranes. This combination of techniques was successful in achieving an approximately 200-fold increase in the activity of the Golgi marker galactan synthase and represents a significant improvement for proteomic analyses of the Golgi from conifers. A total of thirty known Golgi proteins were identified by mass spectrometry including glycosyltransferases from gene families involved in glucomannan and glucuronoxylan biosynthesis. The free flow electrophoresis fractions of enriched Golgi were highly abundant in structural proteins (actin and tubulin) indicating a role for the cytoskeleton during compression wood formation. The mass spectrometry proteomics data associated with this study have been deposited to the ProteomeXchange with identifier PXD000557.     

Combined Effects of Auxin Transport Inhibitors and Cytokinin: Alterations of Organ Development in Tobacco

We have examined the effects of the auxin transport inhibitors1-naphthylphthalamic acid (NPA) and 2,3,5-triiodobenzoic acid(TIBA) on leaf morphogenesis of transgenic Nicotiana tabacum(cv. Xanthi) plants expressing the Agrobacterium tumefacienscytokinin biosynthetic gene, ipt. We have observed the formationof saucer-shaped leaf-like organs at the shoot apex and at lateralbuds. The formation of apical saucer-shaped leaf-like organscan be duplicated by the application of exogenous NPA and cytokininto wild-type tobacco seedlings. We have also observed adventitiousleaf-like organs with altered petiole and blade morphology inthe transgenic plants treated with auxin transport inhibitors.These results suggest that the combination of diminished auxintransport and elevated cytokinin can lead to alterations inleaf development in tobacco. ⁴Present address: Genesis Research and Development Corporation,P.O. Box 50, Auckland, New Zealand     

Exploring the Ultrastructural Localization and Biosynthesis of β(1,4)-Galactan in Pinus radiata Compression Wood

Softwood species such as pines react to gravitropic stimuli by producing compression wood, which unlike normal wood contains significant amounts of β(1,4)-galactan. Currently, little is known regarding the biosynthesis or physiological function of this polymer or the regulation of its deposition. The subcellular location of β(1,4)-galactan in developing tracheids was investigated in Pinus radiata D. Don using anti-β(1,4)-galactan antibodies to gain insight into its possible physiological role in compression wood. β(1,4)-Galactan was prominent and evenly distributed throughout the S2 layer of developing tracheid cell walls in P. radiata compression wood. In contrast, β(1,4)-galactan was not detected in normal wood. Greatly reduced antibody labeling was observed in fully lignified compression wood tracheids, implying that lignification results in masking of the epitope. To begin to understand the biosynthesis of galactan and its regulation, an assay was developed to monitor the enzyme that elongates the β(1,4)-galactan backbone in pine. A β(1,4)-galactosyltransferase (GalT) activity capable of extending 2-aminopyridine-labeled galacto-oligosaccharides was found to be associated with microsomes. Digestion of the enzymatic products using a β(1,4)-specific endogalactanase confirmed the production of β(1,4)-galactan by this enzyme. This GalT activity was substantially higher in compression wood relative to normal wood. Characterization of the identified pine GalT enzyme activity revealed pH and temperature optima of 7.0 and 20°C, respectively. The β(1,4)-galactan produced by the pine GalT had a higher degree of polymerization than most pectic galactans found in angiosperms. This observation is consistent with the high degree of polymerization of the naturally occurring β(1,4)-galactan in pine.The ability to respond to gravitropic stimuli is important for the survival of most terrestrial plants. Arborescent angiosperm and gymnosperm species generate wood with modified properties, called reaction wood, in response to gravitropic stimuli (Timell, 1969, 1986; Du and Yamamoto, 2007). The formation of reaction wood enables the return of bent stems to a vertical orientation. Interestingly, the location and type of the reaction wood deposited in woody gymnosperms and angiosperms generally differs significantly. Gymnosperms respond to gravitropic stimuli by compression wood formation on the underside of leaning stems (Timell, 1986), and arboreal angiosperms generate reaction wood primarily in the form of tension wood on the upper side of inclined stems (Timell, 1969).Compression wood in conifers differs significantly from normal wood in its anatomical, chemical, and physical properties. Typical anatomical features of severe compression wood are short, rounded, and thick-walled tracheids with a prominent band of lignin in the outer S2 layer of the cell wall as well as spiral checks and the absence of an S3 layer (Timell, 1986). Biochemically, compression wood is characterized by high levels of lignin, rich in condensed p-hydroxyphenyl units, as well as reduced cellulose and galactoglucomannan relative to normal wood (Timell, 1986; Nanayakkara et al., 2005; Yeh et al., 2006). Most striking, though, is that β(1,4)-galactan can constitute more than 10% (w/w) of the cell wall material in severe compression wood but is virtually absent in normal wood (Nanayakkara et al., 2005; Yeh et al., 2006). Recent work suggests that β(1,4)-galactan biosynthesis represents an early step in compression wood formation and confirms that its presence is diagnostic for this wood type (Altaner et al., 2007). However, the molecular signal cascades in conifers that lead to the deposition of β(1,4)-galactan are currently not well understood.Immunological studies in conifer species using the monoclonal anti-β(1,4)-galactan LM5 antibody (Jones et al., 1997) indicate that β(1,4)-galactan in compression wood is located in the S1 and outer S2 layers of mature tracheids but is virtually absent from the primary cell walls (Schmitt et al., 2006; Altaner et al., 2007; Möller and Singh, 2007). Instead of β(1,4)-galactan, most conifers contain small amounts of arabinogalactan, a polysaccharide characterized by a highly branched β(1,3)-galactan backbone (Vikkula et al., 1997; Willför et al., 2002; Laine et al., 2004) in their primary cell walls. The ultrastructural distribution of β(1,4)-galactan in compression wood appears to be largely consistent with highly lignified cell wall layers (Möller and Singh, 2007), which might explain the involvement of β(1,4)-galactan in the formation of lignin-carbohydrate complexes (Mukoyoshi et al., 1981; Minor, 1982; Timell, 1986; Laine et al., 2004).The investigation of β(1,4)-galactan structure in preparations from Pinus sylvestris (Laine et al., 2004) and Pinus radiata (Nanayakkara 2007) revealed a linear polymer. In Pinus densiflora Siebold & Zucc., β(1,4)-galactan was found to be slightly branched at positions C2, C3, and C6 (Mukoyoshi et al., 1981). β(1,4)-Galactan in conifers display a high degree of polymerization (DP), which was originally estimated to be in the range of 200 to 300 (Timell, 1986). More recent studies with P. radiata compression wood found the native polysaccharide to have a DP of approximately 380 (Nanayakkara 2007).β(1,4)-Galactan is a very good biochemical marker for compression wood (Altaner et al., 2007), but its physiological role is currently not well understood. Various functions for β(1,4)-galactan in compression wood have been proposed, such as strengthening of the secondary cell wall, absorption of mechanical stresses, and generation of compressive forces (Möller and Singh, 2007). Furthermore, β(1,4)-galactan is also found in tension wood, with a proposed role in cross-linking cellulose microfibrils (Arend, 2008). However, all of those hypotheses on the molecular function of β(1,4)-galactan in reaction wood await experimental verification.Despite substantial efforts to characterize the biosynthesis of this polymer, β(1,4)-galactan biosynthetic enzymes and their corresponding genes are currently unknown (Peugnet et al., 2001; Geshi et al., 2002, 2004; Abdel-Massih et al., 2003; Kato et al., 2003; Ishii et al., 2004; Konishi et al., 2004, 2007; Gorshkova and Morvan, 2006). However, based on other cell wall polysaccharide biosynthetic enzymes, it is likely that the enzymes involved in the biosynthesis of β(1,4)-galactan are either Golgi localized or pass through the Golgi in transit to the apoplastic space (Reyes and Orellana, 2008).To better understand β(1,4)-galactan synthesis in compression wood formation, we sampled both normal wood and severe compression wood from two 6-year-old P. radiata trees, which displayed stark differences in lignin and carbohydrate content and composition. Using these wood samples, new insights into the subcellular localization of β(1,4)-galactan in pine were generated using confocal laser fluorescence microscopy and transmission electron microscopy. An enzyme assay was developed, based on 2-aminopyridine (2AP)-labeled galacto-oligosaccharides as acceptor molecules, which we used to identify and partially purify a robust, microsome-associated, UDP-Gal-dependent β(1,4)-galactosyltransferase (GalT) activity in compression wood that was virtually undetectable in normal wood. Assays of the partially purified GalT revealed that this enzyme has some properties similar to those of previously characterized pectic GalTs, but a marked difference was observed in the size distribution of the enzymatic products.     

S RNase and Interspecific Pollen Rejection in the Genus Nicotiana: Multiple Pollen-Rejection Pathways Contribute to Unilateral Incompatibility between Self-Incompatible and Self-Compatible Species

In self-incompatible (SI) plants, the S locus acts to prevent growth of self-pollen and thus promotes outcrossing within the species. Interspecific crosses between SI and self-compatible (SC) species often show unilateral incompatibility that follows the SI x SC rule: SI species reject pollen from SC species, but the reciprocal crosses are usually compatible. The general validity of the SI x SC rule suggests a link between SI and interspecific pollen rejection; however, this link has been questioned because of a number of exceptions to the rule. To clarify the role of the S locus in interspecific pollen rejection, we transformed several Nicotiana species and hybrids with genes encoding SA2 or SC10 RNase from SI N. alata. Compatibility phenotypes in the transgenic plants were tested using pollen from three SC species showing unilateral incompatibility with N. alata. S RNase was implicated in rejecting pollen from all three species. Rejection of N. plumbaginifolia pollen was similar to S allele-specific pollen rejection, showing a requirement for both S RNase and other genetic factors from N. alata. In contrast, S RNase-dependent rejection of N. glutinosa and N. tabacum pollen proceeded without these additional factors. N. alata also rejects pollen from the latter two species through an S RNase-independent mechanism. Our results implicate the S locus in all three systems, but it is clear that multiple mechanisms contribute to interspecific pollen rejection.     

Proteomic phenotyping of Novosphingobium nitrogenifigens reveals a robust capacity for simultaneous nitrogen fixation, polyhydroxyalkanoate production, and resistance to reactive oxygen species

Novosphingobium nitrogenifigens Y88(T) (Y88) is a free-living, diazotrophic Alphaproteobacterium, capable of producing 80% of its biomass as the biopolymer polyhydroxybutyrate (PHB). We explored the potential utility of this species as a polyhydroxybutyrate production strain, correlating the effects of glucose, nitrogen availability, dissolved oxygen concentration, and extracellular pH with polyhydroxybutyrate production and changes in the Y88 proteomic profile. Using two-dimensional differential in-gel electrophoresis and tandem mass spectrometry, we identified 217 unique proteins from six growth conditions. We observed reproducible, characteristic proteomic signatures for each of the physiological states we examined. We identified proteins that changed in abundance in correlation with either nitrogen fixation, dissolved oxygen concentration, or acidification of the growth medium. The proteins that correlated with nitrogen fixation were identified either as known nitrogen fixation proteins or as novel proteins that we predict play roles in aspects of nitrogen fixation based on their proteomic profiles. In contrast, the proteins involved in central carbon and polyhydroxybutyrate metabolism were constitutively abundant, consistent with the constitutive polyhydroxybutyrate production that we observed in this species. Three proteins with roles in detoxification of reactive oxygen species were identified in this obligate aerobe. The most abundant protein in all experiments was a polyhydroxyalkanoate granule-associated protein, phasin. The full-length isoform of this protein has a long, intrinsically disordered Ala/Pro/Lys-rich N-terminal segment, a feature that appears to be unique to sphingomonad phasins. The data suggest that Y88 has potential as a PHB production strain due to its aerobic tolerance and metabolic orientation toward polyhydroxybutyrate accumulation, even in low-nitrogen growth medium.