ABSTRACT
Since industrialization began, atmospheric CO2 ([CO2]) has increased from 270 to 415 ppm and is projected to reach 800-1000 ppm this century. Some Arabidopsis thaliana (Arabidopsis) genotypes delayed flowering in elevated [CO2] relative to current [CO2], while others showed no change or accelerations. To predict genotype-specific flowering behaviors, we must understand the mechanisms driving flowering response to rising [CO2]. [CO2] changes alter photosynthesis and carbohydrates in plants. Plants sense carbohydrate levels, and exogenous carbohydrate application influences flowering time and flowering transcript levels. We asked how organismal changes in carbohydrates and transcription correlate with changes in flowering time under elevated [CO2]. We used a genotype (SG) of Arabidopsis that was selected for high fitness at elevated [CO2] (700 ppm). SG delays flowering under elevated [CO2] (700 ppm) relative to current [CO2] (400 ppm). We compared SG to a closely related control genotype (CG) that shows no [CO2]-induced flowering change. We compared metabolomic and transcriptomic profiles in these genotypes at current and elevated [CO2] to assess correlations with flowering in these conditions. While both genotypes altered carbohydrates in response to elevated [CO2], SG had higher levels of sucrose than CG and showed a stronger increase in glucose and fructose in elevated [CO2]. Both genotypes demonstrated transcriptional changes, with CG increasing genes related to fructose 1,6-bisphosphate breakdown, amino acid synthesis, and secondary metabolites; and SG decreasing genes related to starch and sugar metabolism, but increasing genes involved in oligosaccharide production and sugar modifications. Genes associated with flowering regulation within the photoperiod, vernalization, and meristem identity pathways were altered in these genotypes. Elevated [CO2] may alter carbohydrates to influence transcription in both genotypes and delayed flowering in SG. Changes in the oligosaccharide pool may contribute to delayed flowering in SG. This work extends the literature exploring genotypic-specific flowering responses to elevated [CO2].
Subject(s)
Arabidopsis , Arabidopsis/metabolism , Carbon Dioxide/metabolism , Genotype , Carbohydrates , Oligosaccharides/metabolism , Sugars/metabolism , Gene Expression Regulation, Plant , Flowers/metabolism , Plant Leaves/metabolismABSTRACT
Altered flowering time at elevated [CO 2 ] is well documented, although mechanisms are not well understood. An Arabidopsis genotype previously selected for high fitness at elevated [CO 2 ] (SG) showed delayed flowering and larger size at flowering when grown at elevated (700 ppm) versus current (380 ppm) [CO 2 ]. This response was correlated with prolonged expression of FLOWERING LOCUS C ( FLC ), a vernalization-responsive floral repressor gene. To determine if FLC directly delays flowering at elevated [CO 2 ] in SG, we used vernalization (extended cold) to downregulate FLC expression. We hypothesized that vernalization would eliminate delayed flowering at elevated [CO 2 ] through the direct reduction of FLC expression, eliminating differences in flowering time between current and elevated [CO 2 ]. We found that with downregulation of FLC expression via vernalization, SG plants grown at elevated [CO 2 ] no longer delayed flowering compared to current [CO 2 ]. Thus, vernalization returned the earlier flowering phenotype, counteracting effects of elevated [CO 2 ] on flowering. This study indicates that elevated [CO 2 ] can delay flowering directly through FLC , and downregulation of FLC under elevated [CO 2 ] reverses this effect. Moreover, this study demonstrates that increasing [CO 2 ] may potentially drive major changes in development through FLC .
ABSTRACT
Conservative flowering behaviours, such as flowering during long days in summer or late flowering at a high leaf number, are often proposed to protect against variable winter and spring temperatures which lead to frost damage if premature flowering occurs. Yet, due the many factors in natural environments relative to the number of individuals compared, assessing which climate characteristics drive these flowering traits has been difficult. We applied a multidisciplinary approach to 10 winter-annual Arabidopsis thaliana populations from a wide climactic gradient in Norway. We used a variable reduction strategy to assess which of 100 climate descriptors from their home sites correlated most to their flowering behaviours when tested for responsiveness to photoperiod after saturation of vernalization; then, assessed sequence variation of 19 known environmental-response flowering genes. Photoperiod responsiveness inversely correlated with interannual variation in timing of growing season onset. Time to flowering appeared driven by growing season length, curtailed by cold fall temperatures. The distribution of FLM, TFL2 and HOS1 haplotypes, genes involved in ambient temperature response, correlated with growing-season climate. We show that long-day responsiveness and late flowering may be driven not by risk of spring frosts, but by growing season temperature and length, perhaps to opportunistically maximize growth.
Subject(s)
Arabidopsis Proteins , Arabidopsis , Humans , Arabidopsis/physiology , Temperature , Arabidopsis Proteins/genetics , Arabidopsis Proteins/metabolism , Seasons , Cold Temperature , Flowers/physiology , Photoperiod , Gene Expression Regulation, Plant , MADS Domain Proteins/geneticsABSTRACT
Temperate species often require or flower most rapidly in the long daylengths, or photoperiods, experienced in summer or after prolonged periods of cold temperatures, referred to as vernalization. Yet, even within species, plants vary in the degree of responsiveness to these cues. In Arabidopsis thaliana, CONSTANS (CO) and FLOWERING LOCUS C (FLC) genes are key to photoperiod and vernalization perception and antagonistically regulate FLOWERING LOCUS T (FT) to influence the flowering time of the plants. However, it is still an open question as to how these genes vary in their interactions among wild accessions with different flowering behaviors and adapted to different microclimates, yet this knowledge could improve our ability to predict plant responses in variable natural conditions. To assess the relationships among these genes and to flowering time, we exposed 10 winter-annual Arabidopsis accessions from throughout Norway, ranging from early to late flowering, along with two summer-annual accessions to 14 weeks of vernalization and either 8- or 19-h photoperiods to mimic Norwegian climate conditions, then assessed gene expression levels 3-, 5-, and 8-days post vernalization. CO and FLC explained both FT levels and flowering time (days) but not rosette leaf number at flowering. The correlation between FT and flowering time increased over time. Although vernalization suppresses FLC, FLC was high in the late-flowering accessions. Across accessions, FT was expressed only at low FLC levels and did not respond to CO in the late-flowering accessions. We proposed that FT may only be expressed below a threshold value of FLC and demonstrated that these three genes correlated to flowering times across genetically distinct accessions of Arabidopsis.
ABSTRACT
We assessed mechanistic temperature influence on flowering by incorporating temperature-responsive flowering mechanisms across developmental age into an existing model. Temperature influences the leaf production rate as well as expression of FLOWERING LOCUS T (FT), a photoperiodic flowering regulator that is expressed in leaves. The Arabidopsis Framework Model incorporated temperature influence on leaf growth but ignored the consequences of leaf growth on and direct temperature influence of FT expression. We measured FT production in differently aged leaves and modified the model, adding mechanistic temperature influence on FT transcription, and causing whole-plant FT to accumulate with leaf growth. Our simulations suggest that in long days, the developmental stage (leaf number) at which the reproductive transition occurs is influenced by day length and temperature through FT, while temperature influences the rate of leaf production and the time (in days) the transition occurs. Further, we demonstrate that FT is mainly produced in the first 10 leaves in the Columbia (Col-0) accession, and that FT accumulation alone cannot explain flowering in conditions in which flowering is delayed. Our simulations supported our hypotheses that: (i) temperature regulation of FT, accumulated with leaf growth, is a component of thermal time, and (ii) incorporating mechanistic temperature regulation of FT can improve model predictions when temperatures change over time.
ABSTRACT
We introduce a cheminformatics approach that combines highly selective and orthogonal structure elucidation parameters; accurate mass, MS/MS (MS²), and NMR into a single analysis platform to accurately identify unknown metabolites in untargeted studies. The approach starts with an unknown LC-MS feature, and then combines the experimental MS/MS and NMR information of the unknown to effectively filter out the false positive candidate structures based on their predicted MS/MS and NMR spectra. We demonstrate the approach on a model mixture, and then we identify an uncatalogued secondary metabolite in Arabidopsis thaliana. The NMR/MS² approach is well suited to the discovery of new metabolites in plant extracts, microbes, soils, dissolved organic matter, food extracts, biofuels, and biomedical samples, facilitating the identification of metabolites that are not present in experimental NMR and MS metabolomics databases.
ABSTRACT
Day length and ambient temperature are major stimuli controlling flowering time. To understand flowering mechanisms in more natural conditions, we explored the effect of daily light and temperature changes on Arabidopsis thaliana. Seedlings were exposed to different day/night temperature and day-length treatments to assess expression changes in flowering genes. Cooler temperature treatments increased CONSTANS (CO) transcript levels at night. Night-time CO induction was diminished in flowering bhlh (fbh)-quadruple mutants. FLOWERING LOCUS T (FT) transcript levels were reduced at dusk, but increased at the end of cooler nights. The dusk suppression, which was alleviated in short vegetative phase (svp) mutants, occurred particularly in younger seedlings, whereas the increase during the night continued over 2 wk. Cooler temperature treatments altered the levels of FLOWERING LOCUS M-ß (FLM-ß) and FLM-δ splice variants. FT levels correlated strongly with flowering time across treatments. Day/night temperature changes modulate photoperiodic flowering by changing FT accumulation patterns. Cooler night-time temperatures enhance FLOWERING BHLH (FBH)-dependent induction of CO and consequently increase CO protein. When plants are young, cooler temperatures suppress FT at dusk through SHORT VEGETATIVE PHASE (SVP) function, perhaps to suppress precocious flowering. Our results suggest day length and diurnal temperature changes combine to modulate FT and flowering time.
Subject(s)
Arabidopsis Proteins/metabolism , Arabidopsis/physiology , DNA-Binding Proteins/metabolism , Flowers/physiology , Gene Expression Regulation, Plant , Transcription Factors/metabolism , Arabidopsis Proteins/genetics , DNA-Binding Proteins/genetics , Photoperiod , Plants, Genetically Modified , Temperature , Transcription Factors/geneticsABSTRACT
Many plants use information about changing day length (photoperiod) to align their flowering time with seasonal changes to increase reproductive success. A mechanism for photoperiodic time measurement is present in leaves, and the day-length-specific induction of the FLOWERING LOCUS T (FT) gene, which encodes florigen, is a major final output of the pathway. Here, we summarize the current understanding of the molecular mechanisms by which photoperiodic information is perceived in order to trigger FT expression in Arabidopsis as well as in the primary cereals wheat, barley, and rice. In these plants, the differences in photoperiod are measured by interactions between circadian-clock-regulated components, such as CONSTANS (CO), and light signaling. The interactions happen under certain day-length conditions, as previously predicted by the external coincidence model. In these plants, the coincidence mechanisms are governed by multilayered regulation with numerous conserved as well as unique regulatory components, highlighting the breadth of photoperiodic regulation across plant species.
Subject(s)
Flowers/growth & development , Gene Expression Regulation, Plant , Genes, Plant , Photoperiod , Plant Leaves/metabolism , Plant Proteins/genetics , Plants/genetics , Arabidopsis Proteins/genetics , Arabidopsis Proteins/metabolism , Circadian Clocks , DNA-Binding Proteins/genetics , DNA-Binding Proteins/metabolism , Flowers/metabolism , Plant Proteins/metabolism , Plants/metabolism , Transcription Factors/genetics , Transcription Factors/metabolismABSTRACT
Photoperiod, or the duration of light in a given day, is a critical cue that flowering plants utilize to effectively assess seasonal information and coordinate their reproductive development in synchrony with the external environment. The use of the model plant, Arabidopsis thaliana, has greatly improved our understanding of the molecular mechanisms that determine how plants process and utilize photoperiodic information to coordinate a flowering response. This mechanism is typified by the transcriptional activation of FLOWERING LOCUS T (FT) gene by the transcription factor CONSTANS (CO) under inductive long-day conditions in Arabidopsis. FT protein then moves from the leaves to the shoot apex, where floral meristem development can be initiated. As a point of integration from a variety of environmental factors in the context of a larger system of regulatory pathways that affect flowering, the importance of photoreceptors and the circadian clock in CO regulation throughout the day has been a key feature of the photoperiodic flowering pathway. In addition to these established mechanisms, the recent discovery of a photosynthate derivative trehalose-6-phosphate as an activator of FT in leaves has interesting implications for the involvement of photosynthesis in the photoperiodic flowering response that were suggested from previous physiological experiments in flowering induction.
ABSTRACT
The plant circadian clock is involved in the regulation of numerous processes. It serves as a timekeeper to ensure that the onset of key developmental events coincides with the appropriate conditions. Although internal oscillating clock mechanisms likely evolved in response to the earth's predictable day and night cycles, organisms must integrate a range of external and internal cues to adjust development and physiology. Here we introduce three different clock outputs to illustrate the complexity of clock control. Clock-regulated diurnal growth is altered by environmental stimuli. The complexity of the photoperiodic flowering pathway highlights numerous nodes through which plants may integrate information to modulate the timing of flowering. Comparative analyses among ecotypes that differ in flowering response reveal additional environmental cues and molecular processes that have developed to influence flowering. We also explore the process of cold acclimation, where circadian inputs, light quality, and stress responses converge to improve freezing tolerance in anticipation of colder temperatures.
Subject(s)
Arabidopsis Proteins/genetics , Arabidopsis/physiology , Circadian Clocks/physiology , Circadian Rhythm/physiology , Flowers/physiology , Gene Expression Regulation, Plant , Adaptation, Physiological , Arabidopsis Proteins/metabolism , Cold Temperature , Light , Photoperiod , Signal TransductionABSTRACT
Reed canary grass (Phalaris arundinacea L.) is a fast-growing, perennial, rhizomatous C3 grass considered as a model invasive species for its aggressive behaviour. The same traits make it a candidate for bioenergy feedstock. We tested the following hypotheses: (1) elevated atmospheric [CO2] and nutrient supply enhance photosynthetic carbon acquisition of this fructan-accumulating grass with little or no photosynthetic downregulation; (2) elevated [CO2] promotes carbon allocation to growth when nutrients are sufficient and to fructan storage in rhizomes when nutrients are low. Plants were grown at ambient or elevated (+320µmolmol-1) [CO2], and fertilised using full or one-eighth strength modified Hoagland solution. We investigated leaf photosynthesis, whole-plant water use, biomass allocation, and nitrogen and carbon storage in rhizomes. Elevated [CO2] enhanced light-saturated net CO2 assimilation by 61%. It doubled whole-plant, stem and root biomass in summer. Plants grown in elevated [CO2] had a greater rate of CO2 assimilation at higher [CO2], indicating a shift in photosynthetic apparatus for enhanced carbon gain under elevated [CO2]. The majority of belowground biomass was allocated to rhizomes for storage rather than to roots in both seasons. In autumn, elevated [CO2] increased fructan concentration in rhizomes from 8.1 to 11.7% of biomass when nutrients were low (P=0.023). Our results suggest that elevated [CO2] combined with sufficient nutrients is likely to enhance carbon gain and growth of P. arundinacea, and to increase its productivity and competitiveness in summer. Elevated [CO2] is likely to enhance long-term fructan storage in rhizomes, which may benefit overwintering and vegetative spread.
