Reversible assembly and amyloidogenesis of the staphylococcal biofilm protein, Aap

Yarawsky, Alexander E.

14 October 2019

No description available.

Biophysics

Staphylococcus epidermidis

accumulation-associated protein

functional amyloid

analytical ultracentrifugation

circular dichroism

intrinsically disordered proteins

Conserved glycine residues control transient helicity and disorder in the cold regulated protein, Cor15a

Sowemimo, Oluwakemi

22 March 2019

COR15A is a cold regulated disordered protein from Arabidopsis thaliana that contributes to freezing tolerance in plants by protecting membranes. It belongs to the (LEA) Late Embryogenesis Abundant group of proteins that accumulate during the later stage of seed development and are expressed in various parts of the plant. During freezing-induced cellular dehydration, COR15A transitions from a disordered structure to a mostly α-helical structure that binds and stabilizes chloroplast membranes when cells dehydrate due to freezing. We hypothesize that increasing the transient α-helicity of COR15A under normal conditions will increase its ability to bind and protect chloroplast membranes when cells are frozen. To test this hypothesis, conserved glycine residues were mutated to alanine to increase α-helicity. NMR spectroscopy was used to examine structural changes of these mutants compared to wildtype in 0% and 20% TFE. The impact of these mutations on the stability of model membranes during a freeze-thaw cycle was investigated by fluorescence spectroscopy. The results of these experiments showed the mutants had a higher content of α-helical secondary structure than wildtype in 0% and 20% TFE. Increased α-helicity of the COR15A mutants improved membrane stabilization during freezing. Altogether, our results suggest the conserved glycine residues are important for maintaining the disordered structure of the protein.

COR15A

Intrinsically disordered proteins (IDPs)

LEA

NMR

Cell Biology

Molecular Biology

Protein Disorder and Dynamics Studied by Molecular Dynamics Simulations and NMR

Yu, Lei

January 2021

No description available.

Chemistry

Biophysics

protein dynamics

intrinsically disordered proteins

IDP

molecular dynamics

MD

NMR

Combining Simulation and the MspA Nanopore to Study p53 Dynamics and Interactions

Schultz, Samantha A

14 November 2023

p53 is a transcription factor and an important tumor suppressor protein that becomes activated due to DNA damage. Because of its role as a tumor suppressor, mutations in the gene that encodes it are found in over 50% of human cancers. The N-terminal transactivation domain (NTAD) of p53 is intrinsically disordered and modulates the function and interactions of p53 in the cell. Its disordered structure allows it to be controlled closely by post-translation modifications that regulate p53’s ability to bind DNA and interact with regulatory binding partners. p53 is an attractive target for developing cancer therapeutics, but its intrinsically disordered region makes it difficult for traditional experimental techniques to resolve its heterogeneous conformational ensemble. This challenge necessitates the use of techniques that can capture the transient structural features and interactions of p53 to aid in designing effective drugs that can modulate and stabilize its activity. Hybrid-resolution (HyRes) II is a coarse-grained molecular dynamics force field that was parameterized specifically to capture the dynamics of IDPs and can give insight into secondary structure propensity and how post-translational modifications affect the structural ensemble of the protein. Nanopore experiments allow for real-time, single-molecule studies of protein dynamics and interactions with binding partners through characteristic changes in the current that passes through the nanopore. Pairing nanopore experiments with simulations can give insight into the molecular detail of IDP ensembles and interactions, revealing a fuller picture of how p53 is controlled in stressed cell conditions and how its structure is affected due to various modifications and small molecules with therapeutic implications. Herein, we show the HyRes II force field can capture the complex, long-range dynamics of the p53 tetramer and provide molecular-level detail of the p53 autoinhibition mechanism, which is enhanced by the phosphorylation of the NTAD. Secondly, we use the MspA nanopore to capture the differences in events of the wild-type NTAD and a cancer-associated NTAD mutant. Lastly, we detect a small molecule binding to the WT NTAD using nanopore sensing. This approach of integrating MD simulations and nanopore experiments can be applied to the study of other IDPs which are prevalent in biology and integral to human health and disease.

Intrinsically disordered proteins

molecular dynamics

nanopore

p53

Biochemistry

Biophysics

Molecular Biology

Electrostatic properties at the interface of p53 Transactivation domain binding

Corrigan, Alexsandra Nikol

25 May 2021

Intrinsically disordered proteins (IDPs) are an abundant class of proteins and protein regions which rapidly change between multiple structures without an equilibrium position. IDPs exist as a series of conformational ensembles of semi-stable conformations that can be adopted based on a hilly landscape of shallow free energy minima. Disordered sequences share characteristic features differentiating them from globular proteins, including low sequence complexity, low occurrence of hydrophobic residues, high polar and charged residue content, and high flexibility. IDPs are commonly involved in regulation in the cell, and frequently function as, or interact with, hub proteins in protein-protein interaction networks, making them an important class of macromolecules for understanding regulatory and other processes. Given their functional importance, these proteins are widely studied. Many analytical techniques are used, though rapid conformational sampling by IDPs makes it difficult to detect many states with NMR or other techniques. Computational approaches such as molecular dynamics are increasingly used to probe the binding and conformational sampling of these proteins, allowing for observation of factors that cannot be observed with traditional analytical methods such as NMR, such as differing conformational ensembles and the dipoles of individual residues. Here, we studied the role of electrostatic interactions in IDP protein-protein interaction using molecular dynamics simulations performed with the Drude-2019 force field (FF), a polarizable model that allows for more accurate representation of electrostatics, an important factor for highly charged systems like IDPs. For this project, a prototypical protein with disordered regions, p53, was simulated with two protein partners, the nuclear coactivator domain of the CREB binding protein (CBP), and the E3 ubiquitin-protein ligase mouse double minute 2 (MDM2). p53 is widely studied, and the p53 transactivation domain (TAD) is disordered and binds to many structurally diverse partners, making this protein domain a useful model for probing the role of electrostatic interactions formed by IDPs at protein-protein binding interfaces. We found that the Drude-2019 FF allows for simulation of the p53 TAD with Cα chemical shifts comparable to those observed with NMR, supporting that the Drude-2019 FF performs well in simulating IDPs. We observed large relative change in sidechain dipole moments when comparing the p53 TAD alone and when bound to either CBP or MDM2. We observed that aliphatic and aromatic amino acids experienced the largest relative change in sidechain dipole moments, and that there is sensitivity to binding shown in this dipole response. The largest percent changes in sidechain dipole moment were found to localize at and around the binding interface. Understanding the binding interactions of IDPs at a fundamental level, including the role of electrostatic interactions, may help with targeting IDPs or their partners for drug design. / Master of Science in Life Sciences / Many proteins adopt one main structure, and these proteins are called ordered proteins. Intrinsically disordered proteins (IDPs) are an abundant category of proteins which adopt multiple structures, and transition between these different structures is based on factors such as the environment around them, modifications, or interactions with other macromolecules. The flexible structures of IDPs allow them to bind to multiple different partners and to regulate processes in the cell. Since IDPs often regulate processes important to cell function, when these proteins are mutated, misfolded, or otherwise mis-regulated the resulting issues are associated with disease states. IDPs are widely studied with analytical techniques, but because IDPs frequently change shape it can be difficult to observe certain behaviors or certain factors with these techniques. Computational approaches, such as molecular dynamics (MD). MD is the study of molecular motion and interaction, and can allow observation of factors that would be difficult or impossible to observe otherwise, such as the varying structures of IDPs or the dipole moments of specific amino acids within the proteins. For this project we wanted to probe the role of dipole moments, which are charge-based interactions, in the binding of IDPs to protein partners, to better understand how IDPs bind to different partners. We used the p53 protein as an example of IDP binding and simulated it alone and bound to two other proteins, the CREB binding protein (CBP), and the E3 ubiquitin-protein ligase mouse double minute 2 (MDM2). We observed that our simulations were comparable to experiments done with nuclear magnetic resonance spectroscopy, which served to validate that our simulations were realistic. We observed that the dipole moments of the proteins change when simulating the proteins alone and in complex, and that the largest relative changes in dipole are observed for regions of the proteins involved in binding. Probing the role of charge-based interactions in protein-protein binding interactions for IDPs can help us to greater understand these interactions at a more fundamental level and could help with targeting IDPs or their partners for drug design or other problems.

Intrinsically disordered proteins

p53 transactivation domain

molecular dynamics

Drude-2019 force field

electrostatic interactions

MDM2

CBP

Strukturní charakterizace vybraných náhodných proteinových sekvencí s vysokým obsahem neuspořádanosti / Structural characterization of selected random protein sequences with high disorder content

Ptáčková, Barbora

January 2018

An infinitesimal fraction of the practically infinite sequence space has achieved enormous functional diversity of proteins during evolution. Intrinsically disordered proteins (IDPs) which lack a fully defined three-dimensional structure are the most likely precursors to today's proteins because of their flexible conformation and functional diversity. But how have these proteins evolved into often rigid and highly specialized protein structures? This evolutionary trajectory has the greatest support in the theory of induced fold whereby the development of the structure was mediated by the interaction and coevolution of primordial unstructured proteins with different cofactors or RNA molecules. Although some random sequences from the sequence space which is not used by nature are also able to form folded proteins the more suitable candidates for evolution of structure and function appear to be random sequences with a high content of disordered which have low aggregation propensity. The selected random protein sequences with high disorder content have been structurally characterized in this work for their further use in evolutionary studies. Three artificial proteins were selected from a random-sequence library based on previous study in our laboratory. In the present work they were purified and...

Etude des états multiples des domaines WH2 en interaction avec l’actine par résonance magnétique nucléaire / Interaction mechanisms of intrinsically disordered WH2 repeats with actin by nuclear magnetic resonance spectroscopy

Deville, Célia

10 July 2015

Les domaines thymosineβ/WH2 sont une famille de protéines intrinsèquement désordonnées impliqués dans le remodelage du cytosquelette d’actine. Ces domaines de 20 à 50 acides aminés existent seuls ou au sein de protéines modulaires, isolés ou répétés. Ils exercent de nombreuses fonctions : ils séquestrent des monomères d’actine, promeuvent l’assemblage du filament, nucléent, fragmentent et coiffent les filaments. Tous les domaines WH2 interagissent de manière similaire avec l’actine via une hélice amphipathique N-terminale suivie d’un brin central et d’une région C-terminal plus ou moins longue et dynamique. Une étude antérieure a montré que la fonction des domaines βT/WH2 isolés était liée à la dynamique du complexe avec l’actine déterminée par une combinaison d’interactions intermoleculaires le long de l’ensemble de la séquence. Les mécanismes expliquant la multifonctionnalité des domaines WH2 répétés restent vagues. Ce travail de thèse présente tout d’abord la production d’actine recombinante, sauvage et mutée dans le système baculovirus/Sf9 pour la biologie structurale ainsi que le développement de stratégies de marquage isotopique en cellules d’insectes. La deuxième partie s’intéresse à la caractérisation structurale et dynamique de domaines WH2 seules en solution : deux domaines isolés et deux protéines contenant deux domaines WH2. Les hélices amphipathiques N-terminales sont partiellement repliées avec des populations variant selon les protéines. La préstructuration des régions C-terminales est plus variable, complètement désordonnée ou partiellement hélicoïdale selon les protéines. La dernière partie présente l’étude de l’interaction de ces protéines avec l’actine. / WH2 domains are a family of intrinsically disordered proteins involved in actin cytoskeleton remodeling. These short domains, isolated or repeated in various actin binding proteins display a low sequence identity and a large panel of functions such as sequestration of actin monomers, promotion of unidirectional assembly, nucleation, fragmentation, filament capping. All WH2 domains fold similarly upon actin binding. They form an extended interface along actin, with an amphipathic N-terminal helix followed by an extended central strand and a more dynamic C-terminal region. Previous work on single βT/WH2 domains showed that function was linked to the dynamics of the complex with actin which is determined by a combination of intermolecular interactions throughout the sequence. The multifunctionality of WH2 tandem repeats is still elusive. The present work first describes production of recombinant wild-type and mutant actin in insect cells and isotopic 15N-labeling for NMR spectroscopy. As a first step to gain insight into the folding upon binding mechanism of functionally different WH2 repeats, we investigated the conformational behavior of two single domains and two tandem repeats free in solution by NMR. The N-terminal amphipatic helix is partially formed but with various propensities depending on the proteins while the C-terminal region that may form an helix in the complex may be either completely disordered or partially formed in absence of actin. Investigation of WH2:actin interaction for the same four proteins is described in the last chapter.

Actine

Domaines WH2

Résonance magnétique nucléaire

Interactions protéines-protéines

Dynamique des protéines

Intrinsically disordered proteins

Actin

540

Régulation d'enzymes du cycle de Calvin-Benson par une protéine intrinsèquement désordonnée, la CP12, chez Chlamydomonas reinhardtii / Regulation of Calvin-Benson cycle enzymes by the intrinsically disordered protein CP12 in Chlamydomonas reinhardtii

Thieulin Pardo, Gabriel

02 December 2015

La phosphoribulokinase (PRK) et la glycéraldéhyde 3-phosphate déshydrogénase (GAPDH) sont deux enzymes-clés du cycle de Calvin-Benson. Leurs activités sont régulées par l’intermédiaire de la CP12, une protéine intrinsèquement désordonnée. Au cours de la transition lumière-obscurité, la GAPDH, la CP12 et la PRK forment un complexe supramoléculaire au sein duquel l’activité des enzymes est inhibée. Dans les travaux présentés ici, nous nous sommes intéressés à la formation de ce complexe et à la dynamique de ses composants. Nous avons montré pour la première fois que les résidus cystéine Cys243 et Cys249 de la PRK sont essentiels à la formation du complexe GAPDH-CP12-PRK et qu’ils peuvent former un pont disulfure en présence de CP12. Nous avons également étudié la dynamique de la CP12 en présence de ses partenaires, et observé que la CP12 adopte une conformation beaucoup plus compacte en présence de GAPDH et de PRK. La glutathionylation (formation d’un pont disulfure mixte entre une molécule de glutathion et un résidu cystéine appartenant à une protéine) est une modification post-traductionnelle associée au stress oxydant qui affecte dix enzymes du cycle de Calvin-Benson, y compris la GAPDH et la PRK. Nous avons étudié l’impact de la glutathionylation sur ces enzymes, et montré que l’inactivation de la PRK naît de l’encombrement du site de fixation de l’ATP.Enfin, la dernière partie de ces travaux est centrée sur l’adénylate kinase 3 de C. reinhardtii, une enzyme impliquée dans le métabolisme de l’ATP et qui possède une extension similaire à la CP12. Cette première étude montre que cette extension augmente la stabilité de l’ADK 3 et intervient dans sa glutathionylation. / Phosphoribulokinase (PRK) and glyceraldehyde 3-phosphate dehydrogenase (GAPDH) are two key enzymes of the Calvin-Benson and their activities are redox-regulated through the intervention of CP12, a intrinsically disordered protein. During the light-to-dark transitions, GAPDH, CP12 and PRK form a supramolecular complex in which the enzymes are strongly inhibited; this complex is dissociated during the dark-to-light transition and the active enzymes are released.In the work presented here, we studied the formation of the complex and the dynamics of its components. For the first time, we showed that two cysteine residues of PRK, Cys243 and Cys249, are essential to the assembly of the GAPDH-CP12-PRK complex, and can form a disulfide bridge in presence of CP12.Glutathionylation (the formation of a mixed disulfide bridge linking one glutathione molecule and a cysteine residue from a protein) is a post-translational modification associated with oxidative stress that affects ten of the Calvin-Benson enzymes, including GAPDH and PRK, and we show that the inactivation of PRK by glutathionylation is caused by the blockage of the ATP binding site by glutathione.The last part of this work is centered around adenylate kinase 3 from C. reinhardtii, an enzyme tied to the energetic metabolism of the cells that presents a CP12-like C-terminal extension. Our results suggest that this CP12-like “tail” improve the stability of ADK 3 and participates in tis glutathionylation.

Métabolisme

Cycle de Calvin-Benson

Régulation redox

Metabolism

Intrinsically disordered proteins

Calvin-Benson cycle

Redox regulation

Structural and dynamic characterization of the Golgi Reassembly and Stacking Protein (GRASP) in solution / Caracterização estrutural e dinâmica da proteína de estruturação e compactação do complexo de Golgi (GRASP) em solução

Mendes, Luis Felipe Santos

07 February 2018

The Golgi complex is an organelle responsible for receiving synthesized cargo from the endoplasmic reticulum for subsequent post-translations modifications, sorting and secretion. A family of proteins named Golgi Reassembly and Stacking Proteins (GRASP) is essential for the correct assembly and laterally tethering of the Golgi cisternae, a necessary structuration to keep this organelle working correctly. The GRASP structure is mainly composed of two regions: an N-terminal formed by two PDZ domains connected by a short loop (GRASP domain) and a non-conserved C-terminal region, rich in serine and proline residues. Although there are now a few crystal structures solved for the N-terminal domain, it is surprising to notice that no information is currently available regarding a full-length protein or even about dynamic and structural differences between the two PDZs in solution, which is the main functional region of this protein. Using a full-length GRASP model, we were capable of detecting the coexistence of regular secondary structures and large amounts of disordered regions. The overall structure is less compact than a regular globular protein and the high structural flexibility makes its hydrophobic core more accessible to solvent. GRASP coexist in a dynamic conformational ensemble of a µs-ms timescale. Our results indicate an unusual behavior of GRASP in solution, closely resembling a class of collapsed intrinsically disordered proteins called molten globule. We report here also the disorder-to-order transition propensities for a native molten globule-like protein in the presence of different mimetics of cell conditions. Changes in the dielectric constant (such as those experienced close to the membrane surface) seem to be the major factor capable of inducing several disorder-to-order transitions in GRASP, which seems to show very distinct behavior when in conditions that mimic the vicinity of the membrane surface as compared to those found when free in solution. Other folding factors such as molecular crowding, counter ions, pH and phosphorylation exhibit lower or no effect on GRASP secondary structure and/or stability. This is the first study focusing on understanding the disorder-to-order transitions of a molten globule structure without the need for any mild denaturing condition. Regarding the PDZs that form the GRASP domain, we observed that GRASPs are formed by a more unstable and flexible PDZ1 and much more stable and structurally well-behaved PDZ2. More than that, many of the unstable regions found in PDZ1 are in the predicted binding pocket, suggesting a structural promiscuity inside this domain that correlates with the functional promiscuity of interacting with multiple protein partners. This thesis presents the first structural characterization of a full-length GRASP, the first model of how GRASPs (or any molten globule-like protein) can be modulated by the cell during different cell functionalities and the first work in the community proving that the established idea that both PDZs are structurally equivalent is not completely right / O complexo de Golgi é um organela responsável pela recepção de carga sintetizada no retículo endoplasmático e por subsequente modificações pós-traducionais, classificação e secreção. Uma família de proteínas chamada Golgi Reassembly and Stacking Proteins (GRASP) é essencial para o correto empilhamento das cisternas e conexões laterais das pilhas do complexo de Golgi, uma estruturação necessária para manter essa organela funcionando corretamente. A estrutura das GRASPs é composta de duas regiões principais: uma extensão N-terminal formado por dois domínios PDZ conectados por um loop (domínio GRASP) e uma região C-terminal não conservada, rica em resíduos de serina e prolina. Embora existam algumas estruturas cristalográficas resolvidas para o domínio N-terminal, é surpreendente notar que não havia nenhuma informação na literatura sobre a construção inteira de um GRASP, ou mesmo um estudo detalhado sobre os PDZs no N-terminal em solução, que é a principal região funcional dessa proteína. Usando um modelo de GRASP em sua construção completa, fomos capazes de detectar a coexistência de estruturas secundárias regulares e grandes quantidades de regiões desordenadas. A estrutura é menos compacta do que uma proteína globular e a alta flexibilidade estrutural torna o seu núcleo hidrofóbico mais acessível ao solvente. GRASPs coexistem em um conjunto conformacional dinâmico numa escala de tempo característico de s-ms. Nossos resultados indicam um comportamento incomum da GRASP em solução, similar à de uma classe de proteínas intrinsicamente desordenadas colapsadas conhecidas como glóbulos fundidos. Nós relatamos também as propensões de transição estrutural do tipo desordem-ordem para uma proteína glóbulo fundido nativa, induzidas pela presença de diferentes miméticos de condições celulares especificas. A mudança na constante dielétrica do meio (como as experimentadas próximas à superfície da membrana biológica) é o principal modulador estrutural, capaz de induzir múltiplas transições desordem-ordem na GRASP, sugerindo um comportamento muito distinto quando em condições que imitam a vizinhança da superfície da membrana em comparação com os encontrados quando livre em solução. Outros fatores de enovelamento, tais como o molecular crowding, contra-ions, pH e a fosforilação exibem efeitos menores (ou nenhum) na estrutura secundária e/ou estabilidade da GRASP. Este é o primeiro estudo focado na compreensão das transições desordem-ordem em uma estrutura do tipo glóbulo fundido sem que houvesse a necessidade de qualquer condição desnaturante. Em relação aos PDZs que formam o domínio GRASP, observamos que as GRASPs são formadas por um PDZ1 mais instável e flexível e um PDZ2 muito mais estável e estruturalmente bem comportado. Mais do que isso, muitas das regiões instáveis encontradas no PDZ1 estão no predito bolsão de ligação, sugerindo uma promiscuidade estrutural dentro desse domínio que se correlaciona com a promiscuidade funcional de interação com múltiplos parceiros proteicos. É apresentado nesta tese a primeira caracterização estrutural de uma GRASP em sua forma completa, o primeiro modelo de como as GRASPs (ou qualquer proteína em forma de glóbulo fundido) pode ser modulada estruturalmente pela célula durante diferentes funcionalidades e o primeiro trabalho na comunidade provando que a estabelecido ideia de que ambos os PDZs são estruturalmente equivalentes não é completamente correta

Espectroscopia

GRASP

GRASP

Intrinsically disordered proteins

Molten Globule

Molten Globule

Proteínas intrinsicamente desordenadas

Spectroscopy

Unconventional protein secretion

Biophysical studies of protein assemblies

Wicky, Basile Isidore Martin

January 2019

Proteins are synthesised as linear polymeric chains. The subtle energetic interplay of interatomic interactions results in chain folding, through which proteins may acquire defined structures. This spatial organisation is encoded by the protein sequence itself; the so-called thermodynamic hypothesis formulated by Anfinsen in 1961. A defined structure is often considered a pre-requisite to protein function, but widespread existence of intrinsically disordered proteins (IDPs) has prompted a re- evaluation of the ways biological function may be encoded into polypeptide chains. Furthermore, proteins often exist as part of multi-component entities, where regulation of assembly is integral to their properties. The interplay between disorder, oligomerisation and function is the focus of this thesis. Some IDPs fold conditionally upon interacting with a partner protein; a process known as coupled folding and binding. What are the biophysical advantages and consequences of disorder in the context of these interactions? A common feature of IDPs is their sequence composition bias, with charged residues being often over-represented. It is therefore tempting to speculate that electrostatic interactions may play a major role in coupled folding and binding reactions. Surprisingly, the opposite was found to be true. Charge-charge interactions only contributed about an order of magnitude to the association rate constants of two contrasting model systems. The lack of pre-formed binding interfaces-a consequence of disorder-might preclude electrostatic acceleration from complementary patches. By looking at the role of the sequence, many studies have taken a protein-centric approach to understanding disorder. Yet there is paucity of data about the effect of extrinsic factors on interactions involving disordered partners. Investigating the role of co-solutes, it was discovered that the kinetic and thermodynamic profiles of coupled folding and binding reactions were sensitive to ion-types. This effect followed the Hofmeister series, and occurred at physiological concentrations of salt. The sensitivity of coupled folding and binding reactions-a consequence of the lack of stability of IDPs-might be advantageous. Given the role of ions in biology, this 'biophysical sensing' could be a mechanism of physiological relevance, allowing modulation of protein-protein interactions involving disordered partners in response to changes in their environments. In cells, signalling networks are often multi-layered, and involve competing protein-protein interactions. The interplay between the biophysical characteristics of the components, and the behaviour of the network were investigated in a model tripartite system composed of folded and disordered proteins. The BCL-2 family regulates the intrinsic pathway of apoptosis through control of mitochondrial outer-membrane permeabilisation; a result of BAK and BAX oligomerisation. Through a shared homology motif (termed BH3), the subtle balance of their interactions determines cellular fate at the molecular level. Characterisation of the model under simple biochemical conditions revealed large differences in affinities among binary interactions; the consequence of the lifetime of the complexes, not their speed of association. A membrane-like environment, re-created using detergents, allows the oligomerisation of BAK and BAX in vitro. Furthermore, investigation of the tripartite system under detergent conditions showed that regulation of the network was the result of competing hetero- and homo-oligomerisation events. Relationships to their biophysical properties were gained by probing their energy landscapes using protein folding techniques. The connection between the biophysical properties of the components of the network and their interactions provides a molecular explanation for the regulation of apoptosis. This thesis offers insights into the ways structured assemblies and environmentally responsive disorder elements may encode functions into proteins.