Carotenoid diversity in novel Hymenobacter strains isolated from Victoria Upper Glacier, Antarctica, and implications for the evolution of microbial carotenoid biosynthesis

Klassen, Jonathan L

11 1900

Many diverse microbes have been detected in or isolated from glaciers, including novel taxa exhibiting previously unrecognized physiological properties with significant biotechnological potential. Of 29 unique phylotypes isolated from Victoria Upper Glacier, Antarctica (VUG), 12 were related to the poorly studied bacterial genus Hymenobacter including several only distantly related to previously described taxa. Further study of these microorganisms revealed genotypic, phenotypic, morphological and chemotaxonomic divergence from named species and suggested that they likely represent novel Hymenobacter species. These studies also indicated, however, that the systematics of Hymenobacter and related microorganisms is more complex than previously realized, and may exhibit poorly defined species boundaries due to cosmopolitan dispersal, significant rates of horizontal gene transfer and reintroduction of archived genotypes, e.g., from glacial ice. These processes are reflected in the carotenoid composition of Hymenobacter and related organisms, which includes several novel methyl- and xylosyl-derivatives of 2'-hydroxyflexixanthin with distributions indicative of horizontal gene transfer or differential gain and/or loss of terminal biosynthetic pathway steps. These processes have been previously underappreciated in assessments of microbial carotenoid diversity and suggest the need for fine-scale phylogenetic study of carotenoid distribution in other microbial taxa. Further comparative genomics-based evaluation of microbial carotenoid biosynthesis indicated its wide phylogenetic distribution and diversification, controlled by several lineage-specific modes of evolution including horizontal transfer, de novo enzyme evolution followed by differential gene loss, co-evolution with biochemically associated structures and elevated mutation rates. The latter especially interacts with horizontal transfer depending on metabolic pathway topology, exemplified by the evolution of purple bacterial carotenoid biosynthesis. Exploration of VUG microbial diversity, therefore, not only revealed novel taxa and biotechnologically interesting compounds but also spurred broader evaluation of the mechanisms of metabolic pathway evolution applicable to many other taxa and biochemical pathways. / Microbiology and Cell Biotechnology

Hymenobacter

Carotenoid

Evolution

Glacier

Horizontal Gene Transfer

Species

2'-hydroxyflexixanthin

FUNCTIONAL ANALYSIS OF GENES CONTROLLING PRODUCTION OF THE LATERAL BRANCHING INHIBITOR IN PEA

Tanya Brcich

Unknown Date

This thesis describes a molecular-based study undertaken to analyse the expression of the RAMOSUS1 (RMS1) and RAMOSUS5 (RMS5) genes in pea (Pisum sativum). Both genes encode carotenoid cleavage dioxygenase (CCD) enzymes that are together proposed to control the synthesis of an inhibitor of bud outgrowth termed SMS (Shoot Multiplication Signal). SMS was recently identified as strigolactone. Expression analyses of RMS1 presented here have built upon earlier experiments which demonstrate it to be a highly regulated transcript. RMS1 mRNA levels are known to be rapidly decreased following removal of the shoot apex but are subsequently restored to that of intact plants by auxin (indole-3-acetic acid or IAA). This regulatory mechanism is retained in all five ramosus mutants tested to date. Together with physiological data, this indicates RMS1, and therefore SMS, are required in IAA-mediated suppression of bud outgrowth. Another significant aspect of RMS1 regulation identified in previous studies involves a graft-transmissible, long-distance feedback signal that moves from shoot to root. This feedback regulation is dependent on the RMS2 gene and enhances RMS1 expression levels. Prior to the cloning of RMS5 and its discovery as a second CCD enzyme in the RMS network, reciprocal grafting studies with the rms mutants indicated RMS5 may act in the same pathway as RMS1 to produce SMS. Multiple studies presented here demonstrate that these two CCD genes are expressed in similar tissues and are regulated by the same signals, specifically IAA and the RMS2-dependent feedback signal. Like RMS1, the RMS5 gene also retains its IAA response in the rms mutants. However, RMS5 is generally less responsive to changes in IAA and RMS2-dependent feedback, as it exhibits smaller fluctuations than RMS1 in its expression levels. Together these findings support a general view that RMS1 is more likely to control a rate-limiting step in SMS synthesis. A previous study indicated that RMS1 expression may be up-regulated by IAA through a posttranscriptional mechanism. This thesis sought to more closely examine the RMS1 and RMS5 IAA response by separately observing the effect of IAA on subsequent transcription. New transcripts, termed heterogenous nuclear RNAs (hnRNAs), were relatively quantified in parallel with existing mRNAs in the steady-state cytoplasmic pool. The experiments conducted here provide further evidence that IAA may act post-transcriptionally to stabilise RMS1 mRNA because the changes in hnRNA are not proportional to the changes in mRNA following IAA-modifying treatments. IAA may still function to induce transcription of RMS1, but this does not appear to be a significant mechanism by which IAA regulates RMS1 expression. In contrast, the IAA induction of RMS5 occurs predominantly via new transcription and RMS5 either lacks or is not as strongly subjected to the IAA-mediated mRNA stabilisation mechanism proposed for RMS1. Initial studies described in this thesis also suggest that IAA could act to regulate the expression of the Arabidopsis orthologues MORE AXILLARY BRANCHING (MAX) genes via a post-transcriptional mechanism. Analyses of MAX hnRNA and mRNA levels in Arabidopsis to date indicate it is the RMS5 orthologue MAX3 which exhibits an IAA response most like RMS1. Additional studies into the regulation of RMS1 and RMS5 presented in this thesis provide further insights into the molecular mechanisms controlling their expression levels. In vitro experiments with the translation inhibitor cycloheximide demonstrate that RMS5 expression levels are increased when protein synthesis is reduced, as previously shown for RMS1. Relative quantification of RMS1 and RMS5 hnRNA levels further demonstrate that the induction by cycloheximide is due primarily to an increase in new transcription, indicating that RMS1 and RMS5 are negatively regulated by a rapidly turned-over transcriptional repressor. Tissue specific effects on RMS1 expression were also observed which are consistent with a protein degradation function of the RMS4 F-box in the shoot. This thesis provides further evidence to suggest that SMS acts in concert with IAA to inhibit the sustained outgrowth of axillary buds. RMS1 and RMS5 expression levels are not regulated by a hypothetical fast decapitation signal which is proposed to cause the initial bud outgrowth occurring prior to decapitation-induced IAA depletion. RMS1, RMS5 and SMS are therefore unlikely to control the initial exit of buds from dormancy to an intermediate transition state. Studies here also suggest that enhanced shoot auxin transport and cytokinin biosynthesis are associated with axillary bud outgrowth because the rms mutants contain elevated shoot expression levels of a gene encoding the auxin efflux carrier PIN1 and two genes controlling cytokinin biosynthesis. Several approaches described in this study were used to characterise the RMS1 and RMS5 proteins. Anti-peptide antibodies were generated against both proteins and the results obtained show that although the antibodies are likely to recognise the full-length proteins, further work is required to effectively detect RMS1 and RMS5 in plant tissues via western blotting. Preliminary in situ immunolocalisation results indicate the RMS1 and RMS5 proteins are localised to the vasculature, consistent with gene expression analyses.

RAMOSUS

bud outgrowth

carotenoid cleavage dioxygenase

auxin

RNA

post-transcriptional

Intracellular Location of Carotenoid Pigments in Yeast-Phase Cells of Wangiella Dermatitidis and Cell Wall Morphology After Enzyme Treatment

Foster, Linda Ann

12 1900

Carotenoid pigments in W. dermatitidis, the first pathogenic, dematiaceous fungus in which carotenoid pigments nave been reported, are located primarily (81%) in lipid organelles which floated on the surface of the supernatant fraction of lysed cells. Pigment in this fraction could be extracted with ethyl ether without prior treatment with acetone indicating the pigment is unbound in the lipid organelle. Eight percent remains after exhaustive ether extraction and is recovered after the sample is treated with acetone indicating this fraction is non-covalently bound to proteins in the membranes associated with the lipid organelle. The remaining pigment (about 12%) represents contamination of the supernatant with the lipid organelles.

Wangiella dermatitidis

carotenoids

carotenoid pigments

intracellular locations

Carotenoids.

Wangiella dermatitidis.

Ultraviolet Radiation Tolerance in High Elevation Copepods from the Rocky Mountains of Colorado, USA

Hudelson, Karista

12 1900

Copepods in high elevation lakes and ponds in Colorado are exposed to significant levels of ultraviolet radiation (UV), necessitating development of UV avoidance behavior and photoprotective physiological adaptations. The copepods are brightly pigmented due to accumulation of astaxanthin, a carotenoid which has photoprotective and antioxidant properties. Astaxanthin interacts with a crustacyanin-like protein, shifting its absorbance from 473 nm (hydrophobic free form, appears red) to 632 nm (protein-bound complex, appears blue). In six sites in Colorado, habitat-specific coloration patterns related to carotenoprotein complex have been observed. The objective of this study was to determine whether pigment accumulation or carotenoprotein expression has a greater effect on resistance to UV exposure. For each site, copepod tolerance to UV was assessed by survivorship during UV exposure trials. Average UV exposure was determined for each habitat. Astaxanthin profiles were generated for copepods in each site. Ability to withstand UV exposure during exposure trials was significantly different between color morphs (p < 0.0001). Red copepods were found to tolerate 2-fold greater levels of UVB than blue or mixed copepods. Additionally, red copepods have much higher levels of total astaxanthin than blue or mixed copepods (p < 0.0001) and receive a higher daily UV dose (p < 0.0003). Diaptomid carotenoprotein sequence is not homologous with that of other crustaceans in which crustacyanin has been characterized which prevented quantification of carotenoprotein transcript expression. Overall, diaptomid color morph may be an important indicator of UV conditions in high elevation lentic ecosystems.

Copepod

ultraviolet radiation

carotenoid

astaxanthin

zooplankton

high elevation lake

β-Carotene 15,15’ Oxygenase-1 (BCO1) and β-Carotene 9,10’ Oxygenase-2 (BCO2) Distribution in Cells From Rat Liver and Intestine

Reed, Vanessa M.

January 2013

No description available.

Nutrition

vitamin A

retinoid

carotenoid

BCO1

BCO2

intestine

liver

Genetic Study of Compositional and Physical Kernel Quality Traits in Diverse Maize (<i>Zea mays</i> L.) Germplasm

Ryu, Si Hwan

January 2010

No description available.

Agriculture

Maize

QTL

selective genotyping

carotenoid

anthocyanin

Arido-America

germplasm

Extraction, Purification and partial Characterization of a Carotenoid Binding Protein (CBP) from the Epidermis of the Monarch Butterfly Larvae (Danaus plexippus)

Fang, Nan

17 June 2016

This dissertation describes the purification and partial characterization of CBP from the epidermis of the monarch butterfly larvae (Danaus plexippus). A yellow protein-carotenoid complex was extracted from the yellow pigmented epidermal tissue from monarch butterfly larvae by homogenization. Additional steps in the purification process included differential precipitation with ammonium sulfate, cation and anion chromatography, and lastly size exclusion chromatography. Polyacrylamide gel electrophoresis demonstrates that a single protein was isolated (M-LBP) having a ~60 kDa molecular weight, the value has subsequently been confirmed by HR-tandem MS. Lutein is the sole carotenoid bound by M-LBP with a stoichiometry of the binding of 2: 1. Immunohistochemistry results show that M-LBP has no cross-reactivity to antibodies for silk worm CBP (Bombix mori) but does have cross-reactivity with antibodies for horn worm epidermal CBP (Agrius convolvuli). Binding affinities were determined using surface plasmon resonance for the carotenoids lutein (KD = 18.6 ± 0.7), R,R-zeaxanthin (KD = 990 ± 60), R,S-zeaxanthin (KD = 60 ± 2). Tryptophyphan fluorescence lifetimes were determined for the apoprotein and compared to those of the native M-LBP. Tryptophan fluorescence lifetimes were found to be 3.9 ns and 3.0 ns, respectively for these two forms of the protein, indicating that upon dissociation of the carotenoid from the protein the tryptophan fluorophore adopts a position where it has less interaction with the polar surface environment.

Carotenoid

carotenoid binding protein

lutein

fluorescence

surface plasmon resonance

Amino Acids, Peptides, and Proteins

Biochemistry

Carbohydrates

Equipment and Supplies

Etude des domaines fonctionnels impliqués dans l'interaction entre la protéine cyanobactérienne photoprotectrice Orange Carotenoid Protein et ses partenaires / Study of Functional domains involved in the interaction between the photoprotective cyanobacterial Orange Carotenoid Protein and its partners

Thurotte, Adrien

30 October 2015

Les cyanobactéries sont des organismes procaryotes photosynthétiques. Si l’énergie leur est essentielle, elle peut également être délétère. Afin de se protéger, elles ont acquis plusieurs mécanismes de photoprotection. La thématique de ma thèse est l’étude de l’un d’entre eux par des approches combinées de biologie moléculaire, biochimie et biophysique.Les antennes collectrices de lumière des cyanobactéries sont des complexes extra-membranaires solubles appelés les phycobilisomes. Ils permettent de canaliser l'énergie vers les centres réactionnels des photosystèmes. Sous forte lumière, l'afflux d’énergie y parvenant crée notamment des espèces réactives de l’oxygène, ce qui est délétère pour la cellule. L’Orange Carotenoid Protein (OCP) est impliquée dans un mécanisme de photoprotection qui diminue l'énergie arrivant au niveau des centres réactionnels en augmentant la part d’énergie dissipée sous forme de chaleur. L’OCP est une caroténo-protéine composée de deux domaines globulaires N- et C-terminal qui lie un caroténoïde. Cette protéine photoactivable est à la fois le senseur, et l’acteur du mécanisme de photoprotection. Le mécanisme est désactivé par une seconde protéine, la FRP (Fluorescence Recovery Protein).Le premier chapitre de ce travail de thèse rapporte l’étude de la spécificité des OCPs isolées chez deux souches différentes pour différentes classes de phycobilisomes dont l’architecture du cœur diffère. Le second chapitre présente la méthode mise au point au laboratoire de production de l’OCP chez E.coli, ainsi que la caractérisation d’OCPs clonées depuis le génome de Synechocystis, A. variabilis et A. platensis et surexprimés chez E. coli. Le troisième présente la structure tridimensionnelle du domaine N-terminal, qui est le domaine effecteur de l’OCP. Dans ce chapitre, nous démontrons que le cofacteur caroténoïde se déplace de 12 angstrom au sein de l’OCP lors de la photoactivation. Le quatrième rapporte que le bras N-terminal de l’OCP est une structure singulière qui maintient la protéine fermée à l’obscurité, évitant que l’OCP ne s’active sous faible lumière, ou à l’obscurité. Le cinquième présente la résolution de la structure et l’identification du site actif de la FRP qui nous ont permis de prédire in silico le site d’attachement putatif de la FRP sur le domaine C-terminal de l’OCP. Dans le chapitre 6, je rapporte que deux résidus, l’aspartate 220 et la phénylalanine 299, sont requis pour que l’activité de la FRP soit maximale, confirmant le site d’interaction prédit. / Cyanobacteria, a photosynthetic prokaryote organism, harvest light for living. But harvesting too much light can be harmful. To protect themselves against this stress, cyanobacteria have developed several photoprotective mechanisms. This manuscript reports my work about one of them by combined technics of molecular biology, biochemistry and biophysics.Cyanobacterial light harvesting antennae are extra-membranous complexes called phycobilisomes. They funnel harvested energy into the photosynthetic reaction centers. Under high light, high energy input induces the formation of reactive oxygen species (ROS), which are harmful in excess. One of the existent photoprotective mechanisms helps to avoid ROS formation by decreasing the energy arriving at the reaction centers. The main actor of this mechanism is the photoactive Orange Carotenoid Protein (OCP) that binds to the phycobilisome, and induces an increase of the part of energy dissipated as heat. The OCP is a protein composed by two globular domains (called N- and C- terminal) and binds a carotenoid cofactor. High intensity of blue-green light triggers conformational changes in the inactive orange OCP, which turns red and is now able to binds the PBs. Under low light conditions, this mechanism is turned off by another protein, the Fluorescence Recovery Protein (FRP).The first chapter of this manuscript reports the study of the specificity of OCPs isolated from two strains for different classes of phycobilisomes with different core architecture. The second describe the development of a method to produce holoOCP in E. coli cells. Furthermore, it reports the characterization of the Synechocystis, A. variabilis and A. platensis OCPs isolated from E. coli. The third chapter presents the tridimensional structure of the active N-terminal domain of the OCP. In this chapter, we demonstrate that the carotenoid undergoes a 12anstrom movement upon photoactivation. The fourth chapter rapports that the N-terminal arm of the OCP helps to maintain closed the inactive orange OCP in darkness or low light, avoiding OCP activation and consequent unwanted PBs fluorescence quenching. The fifth presents the resolution of the structure and the identification of the active site of the FRP. These data allow to compute a predictionnal model of interaction between OCP and FRP. I assessed the validity of the model by isolating several modified OCPs. Results shown in chapter 6 report that the aspartate 220 end the phenylalanine 299 are required for effective FRP action.

Cyanobactérie

Bio chimie

Energie renouvelable

Bio physique

OCP (Orange Carotenoid Protein)

Phycobilisome

Cyanobacteria

Bio chemistry

Renewable energy

Bio physics

OCP (Orange Carotenoid Protein)

Phycobilisome

Étude du mécanisme de photoprotection lié à l’Orange Carotenoid Protein et ses homologues chez les cyanobactéries / Photoprotective mechanism related to the Orange Carotenoid Protein and paralogs in cyanobacteria

Wilson, Flore Adjélé

02 December 2016

La lumière est essentielle pour les organismes photosynthétiques qui convertissent l'énergie solaire en énergie chimique. Cependant, la lumière devient dangereuse lorsque l'énergie qui arrive aux centres réactionnels de l'appareil photosynthétique, est en excès par rapport à l’énergie consommée. Dans ce cas, la chaîne de transport d'électrons photosynthétiques se réduit et les espèces réactives de l'oxygène (ROS) sont accumulées, notamment au niveau des deux photosystèmes, PSI et PSII. Les cyanobactéries ont développé des mécanismes photoprotecteurs qui diminuent l'énergie transférée au PSII atténuant ainsi l'accumulation de ROS et les dommages cellulaires, comme l’extinction non-photochimique (NPQcya) induite par la lumière bleue-verte. La soluble Orange Caroténoïde Protéine (OCPo) est essentielle pour ce mécanisme de photoprotection. L'OCP agit comme un senseur de l’intensité lumineuse et un inducteur de la dissipation d'énergie des phycobilisomes (PBS), l'antenne extra-membranaire des cyanobactéries. L'OCP est la première protéine photo-active à caroténoïde connue comme senseur. Une forte lumière bleue-verte déclenche des changements structurels dans l'OCPo qui induisent une forme active, rouge (OCPr). Le domaine N-terminal de l’OCPr, en s’intercalant entre les trimères externes d’un des cylindres basaux du cœur du PBS, augmente la dissipation thermique de l'énergie au niveau de l'antenne. L'OCP possède aussi une autre fonction : l’extinction de l’oxygène singulet, qui protège les cellules du stress oxydatif. Pour récupérer pleinement la capacité de l’antenne en faible lumière, une deuxième protéine est nécessaire, la "Fluorescence Recovery Protein" (FRP), dont le rôle est de détacher l’OCPr des PBS et d’accélérer sa reconversion en OCPo inactive. Ce manuscrit est un état des lieux des connaissances et des dernières avancées sur le mécanisme de NPQ associé à l'OCP dans les cyanobactéries. / Photosynthetic organisms use light energy from the sun in order to perform photosynthesis and to convert solar energy into chemical energy. Absorbance of excess light energy beyond what can be consumed in photosynthesis is dangerous for these organisms. Reactive oxygen species (ROS) are formed at the reaction centers and collecting light antennas inducing photooxidative damage which can lead to cell death. In cyanobacteria, one of these photoprotective mechanisms consists to reduce the amount of energy arriving to the reaction centers by thermal dissipation of the excess absorbed energy. Energy dissipation is accompanied by a decrease of Photosystem II-related fluorescence emission called non-photochemical quenching (NPQ). The soluble Orange Carotenoid Protein (OCPo) is essential for this photoprotective mechanism. The OCP is the first photo-active protein with a carotenoid known as light intensity sensor and acts as energy quencher of the phycobilisome (PB), the extra-membrane antenna of cyanobacteria. Structural changes occur when the OCPo absorbs a strong blue-green light leading to a red active form (OCPr). The N-terminal domain of OCPr burrows into the two external trimers of the core basal APC cylinders of the PB and increases thermal energy dissipation at the level of antenna. The OCP has an additional function in photoprotection as oxygen singlet quencher protecting cells from oxidative stress. Under low light conditions, to recover the full antenna capacity, a second protein is needed, the "Fluorescence Recovery Protein" (FRP), whose role is to detach the OCPr from the PB and accelerate its conversion into an inactive OCPo. In this manuscript, I will review the knowledge about the OCP, since the discovery of the mechanism and its characterization to the latest advances on the OCP-related-NPQ mechanism in cyanobacteria.

Orange Carotenoid Protein

Cyanobacterie

Photoprotection

Photosynthèse

Quenching non photochimique

Fluorescence Recovery Protein

Phycobilisome

Synechocystis

Orange Carotenoid Protein

Cyanobacteria

Photoprotective

Photosynthesis

Non photochemical quenhing

Fluorescence Recovery Protein

Phycobilisome

Synechocystis

Naturally occurring variation in the promoter of the chromoplast-specific Cyc-B gene in tomato can be used to modulate levels of ß-carotene in ripe tomato fruit

Orchard, Caleb

January 2014

No description available.

Horticulture

Agriculture

Genetics

Plant Sciences

tomato

Solanum lycopersicum

B-carotene

CYC-B

carotenoid

promoter

proVitamin A

carotenoid biosynthesis

allele

marker-assisted backcrossing

background genome selection