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Biochemical and functional analysis of the ubiquitin binding properties of the NF-κB regulator NEMO
(2012)
Posttranslationale Modifikationen regulieren wesentliche Eigenschaften von Proteinen, wie z. B. Lokalisation, Konformation, Aktivität, Stabilität und Interaktionsfähigkeit. Eine besondere Form der Proteinmodifikation ist die Ubiquitylierung, bei der das kleine Protein Ubiquitin mit seinem C-Terminus kovalent an ein Substratprotein gebunden wird.
Die am besten untersuchte Funktion der Ubiquitylierung ist die Markierung eines Substrates für den Abbau durch das Proteasom. In den letzten Jahren wurde jedoch entdeckt, dass Ubiquitylierung in vielen Bereichen der Zelle eine wichtige Rolle spielt. Dazu gehören der Transport von Vesikeln, die Reparatur von DNA-Schäden und zelluläre Signalübertragung. Ubiquitin kann verschieden-artige Ketten bilden, indem ein Ubiquitin an eines der sieben Lysine (K6, K11, K27, K29, K33, K48, K63) oder den N-Terminus eines anderen gebunden wird. Diese unterschiedlichen Kettentypen regulieren verschiedene Prozesse. Z. B. dienen K48-verknüpfte Ubiquitinketten als Signal für den proteasomalen Abbau, wohingegen über K63 verknüpfte Ketten hauptsächlich eine Rolle bei Signalübertragungen spielen.
Die meisten Funktionen die durch Ubiquitylierung reguliert werden, werden durch Ubiquitinrezeptoren vermittelt, die eine Ubiquitinbindedomäne (UBD) besitzen. Manche UBDs binden selektiv nur einen Ubiquitinkettentyp und sind somit in der Lage gezielt Prozesse regulieren zu können, indem sie nur durch diesen speziellen Kettentyp aktiviert werden.
Das Protein NEMO ist ein Ubiquitinrezeptor, dessen UBD UBAN selektiv bestimmte Ubiquitinketten bindet. NEMO spielt eine zentrale Rolle bei der Aktivierung der Transkriptionsfaktorfamilie NF-κB, indem es den IKK-Kinasekomplex reguliert. Dieser Kinasekomplex sorgt durch die Phosphorylierung des NF-κB-Inhibitors IκBα für dessen proteasomalen Abbau, wodurch schließlich NF-κB aktiviert wird. Die NF-κB-Aktivierung kann u. a. durch den TNF-Rezeptor (TNFR) induziert werden. Am aktivierten TNFR werden viele Proteine durch verschiedene Ubiquitinketten modifiziert. Bisher wurde angenommen, dass die spezifische Bindung von NEMO an K63-verknüpfte Ubiquitinketten ausschlaggebend für die Aktivierung von IKK ist. Jedoch spielen lineare Ubiquitinketten, die über den N-Terminus verknüpft sind, auch eine wichtige Rolle bei der Aktivierung von NF-κB und die UBAN von NEMO hat eine sehr hohe Affinität zu linearen Ubiquitinketten.
Um die genauen Vorgänge zu verstehen, die zur Aktivierung von NF-κB am TNFR führen, ist es nötig, zu analysieren, welche Proteine mit welchen Ubiquitinketten modifiziert werden und welche Ubiquitinrezeptoren daran binden.
In dieser Studie sollte detailliert untersucht werden, mit welchen Ubiquitin-ketten NEMO bevorzugt interagiert. Dazu wurden in vitro-Bindungsstudien mit bakteriell aufgereinigtem NEMO und verschiedenen Ubiquitinketten durchgeführt. Des Weiteren sollte geprüft werden, wie die Bindung von NEMO an bestimmte Ubiquitinketten die Aktivierung von NF-κB reguliert.
Dabei ergab sich, dass sowohl NEMO in voller Länge, als auch die UBAN, bevorzugt mit linearen Ubiquitinketten interagieren, wohingegen die Interaktion von NEMO mit anderen Ubiquitinketten relativ schwach ist. Ausgehend von einer Kristallstruktur eines Komplexes aus der NEMO-UBAN und linearem di-Ubiquitin, wurden NEMO-Mutanten generiert, die seletkiv die Bindung von NEMO an lineare Ubiquitinketten verhindern, während die schwache Bindung von NEMO an längere K63-verknüpfte Ketten erhalten blieb. Um die Relevanz der Interaktion von NEMO mit linearen Ubiquitinketten für die Aktivierung von NF κB zu überprüfen, wurden diese NEMO-Mutanten dann verwendet um Zellen die kein NEMO exprimieren zu rekonstituieren. Nach Stimulation dieser Zellen mit TNFα wurde NF-κB kaum aktiviert, womit gezeigt werden konnte, dass NEMO gezielt an lineare Ubiquitinketten binden muss, um NF-κB zu aktivieren. Zusätzlich zu seiner Rolle bei der Aktivierung von NF-κB ist NEMO ein wichtiger Inhibitor der durch den TNFR induzierten Apoptose. In dieser Studie wurde gezeigt, dass diese Apoptoseinhibierung abhängig von der Bindung von NEMO an lineare Ubiquitinketten ist, da die Zellen die NEMO-Mutanten exprimierten, die keine linearen Ketten binden können, durch Apoptose starben, währen Wildtyp-Zellen überlebten.
Zusammenfassend konnte in dieser Studie gezeigt werden, dass NEMO bevorzugt und mit vergleichsweise hoher Affinität an lineare Ubiquitinketten bindet und dass diese spezifische Bindung wichtig für die Inhibierung von TNFR-induzierter Apoptose sowie für die Aktivierung von NF-κB ist.
Protein ubiquitination is a post-translational modification that typically involves the conjugation of ubiquitin to substrate proteins via a three-enzyme cascade and regulates a wide variety of cellular processes. Recent studies have revealed that SidE family of Legionella effectors such as SdeA catalyzes novel phosphoribosyl-linked ubiquitination (PR-ubiquitination) of serines in host substrate proteins utilizing NAD+, without the need of E2, E3. The catalytic core of SdeA comprises a mono-ADP-ribosyltransferase (mART) domain that functions to ADP-ribosylate ubiquitin, and a phosphodiesterase (PDE) domain that processes ADP-ribosylated ubiquitin and transfers the resulting phosphoribosylated ubiquitin to serines of substrates.
To date, extensive efforts have been made to study the function of SdeA and mechanism of SdeA mediated PR-ubiquitination, however, the cellular effects of this novel ubiquitination and phosphoribosylation of ubiquitin remained poorly understood. In our study, using biochemical and cell biological approaches, we explored the biological effect of phosphoribosylation of ubiquitin caused by SdeA in cells. We found that phosphoribosylated ubiquitin is not available for conventional ubiquitination, thereby phosphoribosylation of ubiquitin impairs numerous classical ubiquitination related cellular processes including mitophagy, TNF-α signaling and proteasomal degradation.
The precise temporal regulation of the functions of bacterial effectors during Legionella infection by other effectors with antagonizing activities has been well studied so far. Not surprisingly, PR-ubiquitination catalyzed by SidE family effecters is tightly controlled as well, it has been long known that effector SidJ counteracts the toxicity of SdeA to yeast cells. Interestingly, in an experiment for verifying the activity of SidJ, we found that Legionella lysate lacking SidJ was still able to remove ubiquitin from PR-ubiquitinated substrates. Using biochemical approach we identified DupA and DupB, two Legionella bacterial effectors that specifically reverse the novel serine PR-ubiquitination catalyzed by SdeA. We found that DupA and DupB possess a highly homologous PDE domain that removes ubiquitin from PR-ubiquitinated substrates by cleaving the phosphodiester bond between the phosphoribosylated-ubiquitin and serines of substrates. Catalytically deficient mutant DupA H67A strongly binds to PR-ubiquitinated proteins but not capable of cleaving PR-ubiquitin, using it as a trapping bait we identified over 180 substrates of PR-ubiquitination, including a number of ER and Golgi proteins.
In particular, we found that exogenously expressed SdeA localizes to the Golgi apparatus via its C-terminal region and disrupts the Golgi. We validated the identified potential substrates of SidE effectors and found that SdeA modifies Golgi tethering proteins GRASP55 and GRASP65. Using mass spectrometry analyses we identified four serine targets (S3, S408, S409, S449) of GRASP55 PR-ubiquitinated by SdeA in vitro. Ubiquitination of GRASP55 serine mutant in cells co-expressing SdeA or infected with Legionella was markedly decreased, compared with that of the wild-type GRASP55. In addition, with co-immunoprecipitation analyses we found that SdeA-catalyzed ubiquitination regulates the function of GRASP55. PR-ubiquitinated GRASP55 exhibited reduced self-interaction compared to unmodified GRASP55, expression of GRASP55 serine mutant in cells in part rescued Golgi damage caused by SdeA. Furthermore, our study reveals that Golgi structure disruption caused by SdeA does not result in the recruitment of Golgi membranes to the Legionella-containing vacuoles. Instead, it affects cellular secretory pathway including cytokine secretion in cells.
Taken all together, this work expands the understanding of this unconventional PR-ubiquitination catalyzed by Legionella effectors and sheds light on the functions of PR-ubiquitination by which Legionella regulates the Golgi function and secretion pathway during bacterial infection.
Antimicrobial resistance became a serious threat to the worldwide public health in this century. A better understanding of the mechanisms, by which bacteria infect host cells and how the host counteracts against the invading pathogens, is an important subject of current research. Intracellular bacteria of the Salmonella genus have been frequently used as a model system for bacterial infections. Salmonella are ingested by contaminated food or water and cause gastroenteritis and typhoid fever in animals and humans. Once inside the gastrointestinal tract, Salmonella can invade intestinal epithelial cells. The host cell can fight against intracellular pathogens by a process called xenophagy. For complex systems, such as processes involved in the bacterial infection of cells, computational systems biology provides approaches to describe mathematically how these intertwined mechanisms in the cell function. Computational systems biology allows the analysis of biological systems at different levels of abstraction. Functional dependencies as well as dynamic behavior can be studied. In this thesis, we used the Petri net formalism to gain a better insight into bacterial infections and host defense mechanisms and to predict cellular behavior that can be tested experimentally. We also focused on the development of new computational methods.
In this work, the first realization of a mathematical model of the xenophagic capturing of Salmonella enterica serovar Typhimurium in epithelial cells was developed. The mathematical model expressed in the Petri net formalism was constructed in an iterative way of modeling and analyses. For the model verification, we analyzed the Petri net, including a computational performance of knockout experiments named in silico knockouts, which was established in this work. The in silico knockouts of the proposed Petri net are consistent with the published experimental perturbation studies and, thus, ensures the biological credibility of the Petri net. In silico knockouts that have not been experimentally investigated yet provide hypotheses for future investigations of the pathway.
To study the dynamic behavior of an epithelial cell infected with Salmonella enterica serovar Typhimurium, a stochastic Petri net was constructed. In experimental research, a decision like "Which incubation time is needed to infect half of the epithelial cells with Salmonella?" is based on experience or practicability. A mathematical model can help to answer these questions and improve experimental design. The stochastic Petri net models the cell at different stages of the Salmonella infection. We parameterized the model by a set of experimental data derived from different literature sources. The kinetic parameters of the stochastic Petri net determine the time evolution of the bacterial infection of a cell. The model captures the stochastic variation and heterogeneity of the intracellular Salmonella population of a single cell over time. The stochastic Petri net is a valuable tool to examine the dynamics of Salmonella infections in epithelial cells and generate valuable information for experimental design.
In the last part of this thesis, a novel theoretical method was introduced to perform knockout experiments in silico. The new concept of in silico knockouts is based on the computation of signal flows at steady state and allows the determination of knockout behavior that is comparable to experimental perturbation behavior. In this context, we established the concept of Manatee invariants and demonstrated the suitability of their application for in silico knockouts by reflecting biological dependencies from the signal initiation to the response. As a proof of principle, we applied the proposed concept of in silico knockouts to the Petri net of the xenophagic recognition of Salmonella. To enable the application of in silico knockouts for the scientific community, we implemented the novel method in the software isiKnock. isiKnock allows the automatized performance and visualization of in silico knockouts in signaling pathways expressed in the Petri net formalism. In conclusion, the knockout analysis provides a valuable method to verify computational models of signaling pathways, to detect inconsistencies in the current knowledge of a pathway, and to predict unknown pathway behavior.
In summary, the main contributions of this thesis are the Petri net of the xenophagic capturing of Salmonella enterica serovar Typhimurium in epithelial cells to study the knockout behavior and the stochastic Petri net of an epithelial cell infected with Salmonella enterica serovar Typhimurium to analyze the infection dynamics. Moreover, we established a new method for in silico knockouts, including the concept of Manatee invariants and the software isiKnock. The results of these studies are useful to a better understanding of bacterial infections and provide valuable model analysis techniques for the field of computational systems biology.
By adopting a variety of shapes, proteins can perform a wide number of functions in the cell, from being structural elements or enabling communication with the environment to performing complex enzymatic reactions needed to sustain metabolism. The number of proteins in the cell is limited by the number of genes encoding them. However, several mechanisms exist to increase the overall number of protein functions. One of them are post-translational modifications, i.e. covalent attachment of various molecules onto proteins. Ubiquitin was the first protein to be found to modify other proteins, and, faithful to its evocative name, it is involved in nearly all the activities of a cell. Ubiquitylation of proteins was believed for a long time only to be responsible for proteasomal degradation of modified proteins. However, with the discovery of various types of ubiquitylation, such as mono-, multiple- or poly-ubiquitylation, new functions of this post-translational modification emerged. Mono-ubiquitylation has been implicated in endocytosis, chromatin remodelling and DNA repair, while poly-ubiquitylation influences the half-life of proteins or modulates signal transduction pathways. DNA damage repair and tolerance are example of pathways extensively regulated by ubiquitylation. PCNA, a protein involved in nearly all types of DNA transaction, can undergo both mono- and poly-ubiquitylation. These modifications are believed to change the spectrum of proteins that interact with PCNA. Monoubiquitylation of PCNA is induced by stalling of replication forks when replicative polymerases (pols) encounter an obstacle, such as DNA damage or tight DNA-protein complexes. It is believed that monoubiquitylation of PCNA stimulates the exchange between replicative pols to one of polymerases that can synthesize DNA across various lesions, a mechanism of damage tolerance known as translesion synthesis (TLS). Our work has helped to understand why monoubiqutylation of PCNA favours this polymerase switch. We have identified two novel domains with the ability to bind Ub non-covalently. These domains are present in all the members of Y polymerases performing TLS, and were named Ub-binding zinc finger (UBZ) (in polη and polκ) and Ub-binding motif (UBM) (in polι and Rev1). We have shown that these domains enable Y polymerases to preferentially gain access to PCNA upon stalling of replication, when the action of translesion polymerases is required. While the region of direct interaction between Y pols and PCNA had been known (BRCT domain in Rev1 and PIP box motif (PIP) in three others members), we propose that Ub-binding domains (UBDs) in translesion Y pols enhance the PIP- or BRCT-domain-mediated interaction between these polymerases and PCNA by binding to the Ub moiety attached onto PCNA. Following these initial studies, we have also discovered that Y polymerases themselves undergo monoubiquitylation and that their UBDs mediate this modification. This auto-ubiquitylation is believed to lead to an intramolecular interaction between UBD and Ub attached in cis onto the UBD-containing protein. We have mapped monoubiquitylation sites in polη in the C-terminal portion of the protein containing the nuclear localization signal (NLS) and the PIP box. Beside PIP, the NLS motif is also involved in direct interaction of polη with PCNA. Based on these findings, we propose that monoubiquitylation of either NLS or PIP masks them from potential interaction with PCNA. Lastly, using several functional assays, we have demonstrated the importance of all these three motifs in the C-terminus of polη (UBZ, NLS and PIP) for efficient TLS. We have also constructed a mimic of monoubiquitylated polη by genetically fusing polη with Ub. Interestingly, this chimera is deficient in TLS as compared to the wild-type protein. Altogether, these studies demonstrate that the C-terminus of polη constitutes a regulatory module involved in multiple-site interaction with monoubiquitylated PCNA, and that monoubiquitylation of this region inhibits the interaction between polη and PCNA. Our work has also revealed that the UBDs of Y pols as well as of other proteins implicated in DNA damage repair and tolerance, such as the Werner helicase-interacting protein 1 (Wrnip1), are required for their proper sub-nuclear localization. All these proteins localize to discrete focal structures inside the nucleus and mutation of their UBDs results in inability to accumulate in these foci. Interestingly, by exchanging UBDs between different proteins we have learned that each UBD seems to have a distinct functional role, surprisingly not limited to Ubbinding ability. In fact, swapping the UBZ of Wrnip1 with the UBM of polι abolished the localization of Wrnip1 to foci despite preserving the Ub-binding ability of the chimeric protein. In summary, this work provides an overview of how post-translation modification of proteins by Ub can regulate several DNA transactions. Firstly, key regulators (e.g. PCNA) can be differentially modified by Ub. Secondly, specialized UBDs (e.g. UBM, UBZ) embedded only in a subset of proteins act as modules able to recognize these modifications. Thirdly, by means of mediating auto-ubiquitylation, UBDs can modulate the behaviour of host proteins by allowing for either in cis or in trans Ub-UBD interactions.
Clathrin-mediated endocytosis (CME) involves spatially and temporally restricted molecular dynamics.
Although protein kinases and the actin cytoskeleton contribute to the process, whether and how
functions of kinases and actin are integrated remains unknown. Here, we demonstrate that neural
Wiskott-Aldrich syndrome protein (N-WASP) and protein kinase CK2 form a complex and localize on
clathrin-coated vesicles (CCVs). N-WASP binds to and is phosphorylated by CK2, thereby reducing the
kinase activity of CK2. By contrast, N-WASP-promoted actin polymerization is decreased upon both
phosphorylation and binding of CK2. Knockdown of N-WASP and CK2, alone or in combination, results
in impaired endocytosis of epidermal growth factor (EGF) and increased cell-surface levels of EGF
receptor (EGFR). In order to rescue the phenotype of N-WASP-CK2 knockdown cells, both N-WASP and
CK2 activities and abilities to assemble in a complex are required. In summary, this study shows that the
N-WASP-CK2 complex integrates in a single circuit different activities contributing to CME of EGFR and
that the interplay between the two proteins optimizes this process.
Signal-dependent regulation of actin dynamics is essential for many cellular processes, including directional cell migration. In particular, cell migration is initiated by lamellipodia, actin-based protrusions of the plasma membrane. The formation of these protruding structures require incessant assembly and disassembly of actin filaments. The Arp2/3 complex and WAVE proteins are essential for both lamellipodium formation and its dynamics. WAVEs mediate the activation of the Arp2/3 complex downstream of the small GTPase Rac, thus being critical for Rac- and RTK-induced actin polymerization and cell migration. The WAVE-family proteins are always found associated with multiprotein complexes. The most abundant WAVE-based complex is referred to as the WANP (WAVE2-Abi-1-Nap1-PIR121) complex. IQGAP1 is a huge scaffolding protein with multiple protein-interacting domains. IQGAP1 participates in many fundamental activities, including regulation of the actin cytoskeleton, mitogenic, adhesive and migratory responses, as well as in cell polarity and cellular trafficking. IQGAP1 binds to N-WASP, thus raising the possibility that it might control actin nucleation by the Arp2/3 complex. In this study, IQGAP1 was found co-immunoprecipitated not only with WAVE, but also with the endogenous WANP-complex subunits. Correspondingly, IQGAP1 associated to both anti-WAVE and anti-Abi-1 immuno-complexes. Pull-down experiments proved that IQGAP1 binds directly to the WANP-complex subunits. Physical interaction between IQGAP1 and the reconstituted WANP complex could also be demonstrated. Together, these data indicate that IQGAP1 is an accessory component of the WANP complex. Interestingly, the IQGAP-WANP complex disassembled after either EGF stimulation or transfection with constitutively active Cdc42 and Rac1. HeLa cells devoid of IQGAP1 showed diminished and less persistent ruffling upon EGF, but not HGF, stimulation in comparison with the control. This phenotype was accompanied by a strong reduction in chemotaxis towards both growth factors, which was as dramatic as in WANP-complex knockdown (KD) cells. Moreover, GM130 and Giantin showed a polarized and flat ribbon-like pattern in control cells, as it is expected for cis- and cis/medial-Golgi markers. Conversely, small and dispersed vesicular structures were found in both IQGAP1 KD and WANP-complex KD cells. Importantly, Arp2/3-complex silencing resulted in the same phenotypes. Consistently, Brefeldin A-induced disassembly of the Golgi strongly inhibited the IQGAP1-WANP-complex interaction and chemotaxis towards EGF in wild-type cells. The re-expression of an RNAi-resistant wild-type IQGAP1 in IQGAP1 KD cells fully rescued both the ruffling abilities and Golgi structure. A constitutively active mutant, unable to bind to neither Rac1 /Cdc42 nor the WANP complex, could reconstitute only the former defect. Hence, this study shows that actin dynamics regulated by the IQGAP1-WANP complex controls Golgi-apparatus architecture and its contribution to cell chemotaxis. The working model here proposes that at the Golgi apparatus, recruitment of the WANP complex by IQGAP1 leads to the assembly of actin filaments required to maintain the appropriated Golgi morphology. The dissociation of the complex may be required to allow the remodeling of the Golgi membranes in order to respond following a chemoattractant gradient.
Ubiquitin is a highly conserved protein involved in several cellular processes like protein degradation, endocytosis, signal transduction and DNA repair. The discovery of ubiquitin-like proteins (UBL) and ubiquitin-like domains (ULD) increases the number of regulation pathways where the property of the ubiquitin-fold is profitable.
Autophagy is the catabolic pathway used in cells to deliver cytosolic components and dysfunctional organelles to the lysosome for degradation. MAP1LC3 proteins are ubiquitin-like proteins involved in one hand for the expansion of the autophagosome, which sequesters cytosolic substrates. In the other hand, these proteins (LC3- and GABARAP- subfamilies) bind to autophagic receptors linked to polyubiquitinated proteins aggregates. For this project, the 3D structure of the GABARAPL-1/NBR1-LIR complex was determined and confirmed that GABARAPL-1 belongs to the MAP1LC3 proteins family, structurally characterized by an ubiquitin-fold, consisting of a central beta-sheet formed by four beta-strands and two alpha-helices on one side of the beta-sheet, preceded N terminally by two alpha-helices, resulting in the formation of two hydrophobic pockets, hp1 and hp2. The autophagic receptor NBR1 interacts with GABARAPL-1 through the hp1 and hp2 with its LIR motif taking an extended beta conformation upon binding, forming an intermolecular beta-sheet with the second beta-strand of GABARAPL 1. This LC3- interacting region (LIR) consists of an Theta XX Gamma sequence preceded by acidic amino acids, with Theta and Gamma represented by any aromatic and hydrophobic residues, respectively. Interaction studies of the LIR domains of p62, Nix and NBR1 with different members of the MAP1LC3 proteins family indicate that the presence of a tryptophan in the LIR motif increases the binding affinity. Substitution to other aromatic amino acids or increasing the number of negatively charged residues at the N-terminus of the LIR motif, however, has little effect on the binding affinity due to enthalpy-entropy compensation, suggesting that effector proteins can interact with a wide variety of different sequences with similar and moderate binding affinities.
Additionally to be present in proteins dealing with protein folding and degradation, ubiquitin-like domain were found protein involved in the regulation of signal transduction like TBK1, a serine/threonine kinase responsible for induction of immune response. In this second project, based on the NMR chemical shifts of the TBK1 domain contained between amino acids 302 and 383, secondary structure prediction programs (TALOS and CSI) confirmed the presence of an Ubiquitin-like domain in TBK1 by identifying one alpha-helix and four beta-strands sequentially aligned like following beta-beta-alpha-beta-beta. This alignment corresponds perfectly with the secondary structure elements of Ubiquitin and proved that TBK1_ULD belongs to the UBL protein superfamily. The similarity to ubiquitin was even bigger by the presence in addition of a small beta-strand and a short helix, which are observed as the beta 5-strand and a 310-helix in Ubiquitin, respectively. The first attempts on the 3D structure determination confirmed the Ub-fold but due to the lack of assignment in TBK1_ULD, only a structure based on ubiquitin as a model was determined. Interaction studies of TBK1_ULD with the IAD-SRR domain of IRF3 showed that both side of the molecule seems involved and that the TBK1/IRF3 interaction is more complex than a one to one binding process. Unfortunately, the instability of TBK1_ULD associated to the difficulty in the purification of IAD-SRR did not allow to further study this interaction more precisely.
Finally, to overcome the difficulty encountered in NMR experiments because of low expression and/or poor solubility, an expression vector using the intrinsic property of ubiquitin was designed. Fused to proteins or peptides targets, this construct produced proteins and peptides in a larger amount than with traditional expression vectors and also with a less cost than chemical synthesis for pure labeled peptides for NMR structural studies. The presence of a hexa histidine tag was useful for the isolation and the purification of the constructs. The existence of a TEV cleavage site was created to keep the possibility of releasing the ubiquitin moiety from the expressed protein or peptide. Moreover, the ubiquitin-tag could also still be attached to the protein/peptide of interest when biophysical methods like NMR, ITC or CD spectroscopy are applied, providing the same results than for the protein/peptide moiety alone.
Characterization of SPRTN, the first mammalian metalloprotease that repairs DNA-protein-crosslinks
(2019)
DNA is constantly exposed to various endogenous and exogenous sources causing different kinds of DNA damage. To overcome this threat, cells have evolved various repair mechanisms. Impairments of these repair mechanisms result in diverse diseases. Ruijs-Aalfs syndrome is a monogenic disease characterized by accelerated ageing and carcinogenesis, typical features of impaired DNA repair and was shown to be caused by germline mutations of SPRTN, a newly identified and only partially understood protein. A role of SPRTN in DNA damage response was previously shown and an involvement in translesion synthesis (TLS) proposed. However, later discoveries revealed an essential function of SPRTN, being indispensible for embryonic development of vertebrates and cellular survival, whereby this function is independent of SPRTN’s proposed function in TLS. The essential function of SPRTN was proposed to be contained in its protease domain but remained unclear.
In this study we identify SPRTN as the first mammalian metalloprotease that repairs DNA-protein-crosslinks (DPCs). DPCs represent a specific type of DNA-lesions with bulky protein adducts covalently linked to DNA thereby being highly toxic as they potentially stall replication forks and lead to double strand breaks and genomic instability. DPC-repair remains only partially understood despite their frequent appearance and toxicity. With this study we discover and characterize a new mechanism of DPC-repair in mammalian cells - a proteolytic cleavage of the protein adduct by the metalloprotease SPRTN. Accordingly, a proteolytic activity of SPRTN is demonstrated and s SPRTN-recruitment to DNA upon DPC-induction displayed. Furthermore, SPRTN exhibits degradation of different proteins covalently bound to DNA in form of DPCs, but not of unbound fractions of the same protein substrates. Consequently, mutations of SPRTN’s proteolytic core as well as a mislocalization or depletion of SPRTN result in impaired DPC-repair. The importance of SPRTN-mediated DPC-removal is confirmed by a severely compromised response to DPC-inducing agents for cells with impaired SPRTN function. Additionally to the discovery of SPRTN’s essential function this study further provides an explanation of the molecular mechanism underlying Ruijs-Aalfs syndrome (RJALS), the segmental progeroid syndrome resulting from SPRTN mutation. The effects of the identified clinical mutations on the DPC-repair function of SPRTN are explained and a DPC-accumulation in cells carrying clinical SPRTN-mutation displayed. The obtained data provides sufficient evidence that an impaired DPC-repair is the pathophysiologic cause of RJALS-syndrome, confirming the importance of SPRTN’s newly identified function. In conclusion, SPRTN is the first identified mammalian metalloprotease with a DPC-repairing function and the impairment of SPRTN-mediated DPC-removal is the underlying mechanism of RJALS syndrome.
Molecular signaling networks, organized in discrete subsets of proteins in space and time, represent the major principle by which the cell achieves its functional specificity and homeostasis. Complex network organization is preserved by numerous mechanisms, including sequestration of proteins into specific subcellular compartments (eg. organelles), post-translational modifications and most importantly by balanced timing of their biosynthesis and turnover. Two routes of protein degradation, which are fundamentally quite different, are proteasomal and lysosomal-mediated destruction. The latter not only governs degradation of molecules that passed through endocytic or secretory process (trafficking from plasma membrane or Golgi compartment), but also the degradation of cytoplasmic molecules that have been sequestered by a process called macroautophagy (henceforth autophagy). Recently our understanding of autophagic regulatory mechanisms has increased significantly, as molecular details of how autophagy contributes to the degradation of proteins (old, misfolded or aggregated), damaged organelles or pathogens have been deciphered. Initially described as bulk, nonspecific membrane sequestration process induced primarily by nutrient deprivation, autophagy is now known to be selective in terms of cargo recognition and integration into dynamic cellular membrane trafficking system.
My work has addressed the fundamental question of how small ubiquitin-like modifiers LC3/GABARAP, that are conjugated to the autophagic membranes, function within the process of cargo selection and crosstalk between autophagic and endocytic membrane trafficking events. We have employed an initial yeast twohybrid screen to identify LC3/GABARAP interacting partners. Using this technique, we have identified several novel autophagy receptor proteins, mitochondrial protein Nix (BNIP3L), and adaptor proteins, including Rab GTPase activating proteins (TBC family of proteins). Through a conserved LC3 interacting region (LIR), Nix, Rab GAPs and other autophagy adaptor/receptor molecules share a common mode of binding to LC3/GABARAP. However, in contrast to Nix, which specifically facilitates removal of mitochondria in maturing erythrocytes, Rab GAP proteins preferably regulate the dynamics of autophagosome formation and maturation as well as sorting of cargo. Fourteen out of 36 screened Rab GAPs interacted with LC3/GABARAPs. Importantly, identified Rab GAPs are clustered in different regulatory nodes according to the conservation of their GAP domain hence they impact various cellular membrane compartments and organelles, marked by specific subsets of small Rab GTPases. Identification of Rab GAPs that are directly involved in autophagy via binding to LC3 was the first report that clearly pointed to a broader implication of autophagy in all aspects of cellular membrane trafficking. Currently, only few of Rab GAPs are studied in context of autophagy regulation, while large number of them requires further functional characterization.
I have identified two LIR motifs in TBC1D5, Rab7 GAP. LIR1 has also the ability to interact with retromer complex subunit, Vps29. Using several functional assays I have shown that this motif, as well as catalytic Arg within GAP domain are particularly important for function of TBC1D5 in retrograde transport of CI-M6PR from endosomes to the trans-Golgi network (TGN). I have also shown that TBC1D5 binds to LC3 and Vps29 in mutually exclusive way and that Thr at the position 1 and Phe at position 5 of LIR1 motif are both required for TBC1D5 interaction with Vps29. Upon autophagy induction TBC1D5 dissociates from retromer, and associates with autophagic vesicles, while silencing of TBC1D5 significantly impairs autophagic flux. These findings led to the hypothesis that LIR interacting surface on TBC1D5 acts as molecular switch for dual function of TBC1D5. This also indicated that similar surfaces for LIR interaction (similarly to ubiquitin-like domains) are present on proteins other than LC3, and pointed to a dual functionality of the LIR sequence within both endocytic and autophagic pathways.
Following these initial studies, I have also shown that TBC1D5 interacts with AP2 complex subunit AP2M1, and that this interaction plays critical role in TBC1D5-dependent trafficking of Atg9. It is known that Atg9, the only trans-membrane autophagic protein, plays essential role in initiation of autophagy and growth of nascent phagophore membranes. However, machinery that specifically recruits Atg9 traffic carriers to the site of autophagosomes was not known. I subsequently demonstrated that TBC1D5 associates not only with LC3, but also with Atg9 traffic carriers and major initiatory kinase ULK1 during autophagy, while retromer failed to do so. Association of TBC1D5 with Atg9 was dependent on presence of AP2 complex, and on functional clathrin-mediated endocytosis (CME). Based on these and previous findings, model was proposed, that upon induction of autophagy TBC1D5 re-routes Atg9-containing clathrin vesicles from plasma membrane to the site of autophagosome. This led us to the better understanding of TBC1D5 function, but also to the first molecular cue that Atg9 traffics within clathrin-coated vesicles (CCVs). In fact, mutation of Leu-Leu motif within N terminus of Atg9, that potentially mediates interaction with adaptor protein complexes, led to enrichment of Atg9 on plasma membrane and in TGN. This suggested that the sorting motif could be important for interaction of Atg9 with AP2 and AP1 complex, as well. More importantly, TBC1D5 and Atg9 could be directly involved in dynamic regulation of growth factor receptor sorting during autophagy, thus explaining vital role of autophagy in organism development and pathogenesis.
In summary, the work contained within my thesis provides data on the mechanism by which autophagy adaptor proteins participate in cargo selection and regulation of trafficking during autophagy. Firstly, the LIR motif can target proteins or organelles for autophagic degradation (eg. Nix). Secondly, specific LIR motifs can play essential function in recruiting membrane trafficking regulatory proteins that subsequently facilitate phagophore expansion (eg. TBC1D5). Thirdly, by means of reorganization of different protein assemblies (eg. TBC1D5-VPS29 vs. TBC1D5-LC3-Atg9), dynamics of membrane remodeling mediated by Rab GTPases is kept in control during autophagy, thus keeping the organelle integrity and balance within cellular lipid sources unaffected.
NOSTRIN belongs to the recently defined F-BAR protein family. F-BAR proteins are
multi-domain proteins, which serve as adaptors between plasma membrane and
cytoskeleton components in processes such as membrane protrusion formation,
endocytosis and migration. NOSTRIN encompasses a F-BAR domain at the N-terminus,
which mediates membrane association, followed by a HR1 motif and an intermediate
domain (ID) domain in the middle, and a SH3 domain at the C-terminus. The domain
architecture and ability to form oligomers enable NOSTRIN to coordinate several
interaction partners namely dynamin, caveolin, N-WASP and endothelial nitric oxide
synthase (eNOS) in the process of eNOS trafficking. In this context NOSTRIN was
originally identified and hence termed eNOS traffick inducer. NOSTRIN is expressed in
vascularized tissues (e.g. liver and lung) and in primary endothelial cells.
Aims of the present work were (1) to investigate if NOSTRIN is involved in other
processes besides eNOS trafficking, (2) to analyse the function of NOSTRIN in vivo
through knockdown of NOSTRIN in developing zebrafish and (3) to study the
consequences of the loss of NOSTRIN on signal transduction in a primary cell culture
model derived from NOSTRIN knockout mice.
To study the possible involvement of NOSTRIN in other processes besides eNOS
trafficking a yeast two-hybrid screen was performed in which fibroblast growth factor
receptor 1 (FGFR1) was identified as a putative novel interaction partner of NOSTRIN. In
a series of yeast two-hybrid, pulldown and co-immunoprecipitation experiments the
interaction between NOSTRIN and FGFR1 was confirmed to occur between
endogenously expressed proteins and determined to be direct and to depend on the ID
domain of NOSTRIN and the 130 C-terminal amino acid residues of FGFR1. FGFR1 is
activated by binding of fibroblast growth factors (FGFs) and induces several different
signal transduction pathways (e.g. MAPK and Akt pathway). Overexpression of
NOSTRIN in HeLa cells specifically enhanced FGF2-dependent MAPK activation.
Accordingly, depletion of NOSTRIN attenuated FGF2-dependent MAPK activation and
did not affect FGF2-induced Akt activation.
In summary, NOSTRIN has been identified as a novel interaction partner of FGFR1
involved in FGF2-dependent signal transduction.
The morpholino oligonucleotide-mediated knockdown of NOSTRIN in developing
zebrafish caused vascular leakage and irregular vascular patterning e.g. a loss of the
proper trajectory of intersegmental vessel and interruptions of the dorsal longitudinal
anastomotic vessel. The vascular phenotype was consistent upon use of two different
morpholinos and could be rescued in a dose dependent manner by the injection of
zebrafish NOSTRIN mRNA. Detailed analysis involving confocal and time lapse
microscopy in zebrafish with endothelial specific expression of EGFP revealed that the
knockdown of NOSTRIN impacts in vivo on the migration and morphology of endothelial
tip cells and leads to a reduction of filopodia number and length.
Additionally a NOSTRIN knockout mouse was generated. The analysis of FGFR1 signal
transduction in primary mouse lung endothelial cells (MLECs) from NOSTRIN knockout
and wild type mice revealed that FGF2-dependent MAPK activation was attenuated in
MLECs isolated from NOSTRIN knockout mice when compared to MLECs isolated from
wild type mice. The effect of NOSTRIN on FGF2-dependent signal transduction seems to
be specific, since VEGF-induced MAPK activation was not affected in NOSTRIN
knockout MLECs. The importance of NOSTRIN for FGF2 signal transduction in vivo is
demonstrated by the greatly impaired angiogenic response to FGF2 in NOSTRIN
knockout mice in matrigel plug assay. In a detailed biochemical analysis it was
discovered that NOSTRIN interacts with the activated small GTPase Rac1 and that
overexpression of NOSTRIN enhances Rac1 activation. Furthermore, the interactions of
NOSTRIN with both Rac1 and its GEF Sos1 are required for NOSTRIN-mediated
activation of Rac1. In accordance, activation of Rac1 was not detected upon FGF2
stimulation in NOSTRIN knockout MLECs.
In conclusion, the present work describes a novel function of the F-BAR protein
NOSTRIN in FGFR1 signal transduction. Data presented in this work demonstrate that
NOSTRIN is required for the assembly of a complex consisting of FGFR1, Sos1 and
Rac1 and subsequently for the FGF2-dependent activation of Rac1 in endothelial cells.
In Deutschland werden jährlich gut drei Millionen Erythrozytenkonzentrate (EKs) transfundiert. Moderne Herstellungsmethoden und molekulare Diagnoseverfahren konnten die Sicherheit von Blutprodukten im Laufe der Jahre weiter verbessern. Wie bei jedem Medikament kann es nichtsdestotrotz bei der Therapie mit EKs zu Nebenwirkungen kommen. Dazu gehören unter anderem allergische Reaktionen, hämolytische und nicht hämolytische Transfusionsreaktionen, Übertragungen von Infektionskrankheiten und Eisenüberladung. Es werden weitere Nebenwirkungen postuliert, deren Zusammenhang mit Hämotherapie allerdings hinsichtlich einer möglichen Kausalität noch nicht abschließend untersucht wurde. Im Hinblick auf Malignompatienten zeigen retrospektive Untersuchungen eine deutliche Assoziation von Transfusionen und ungünstigem Behandlungsausgang. Diese Beobachtung könnte kausal oder durch Störfaktoren wie den medizinischen Umständen einer Transfusion oder patienteneigener Risikofaktoren erklärt werden. Während randomisierte Studien zur Überprüfung einer Kausalität sich aus ethischen Gründen verbieten, wurden mögliche Mechanismen aufgedeckt, die diese Assoziation erklären könnten. Dazu gehört unter anderem die transfusion-related immunomodulation (TRIM), an der auch erythrozytäre Mikropartikel (red blood cell-derived microparticles, RMPs) beteiligt sein könnten.
RMPs sind extrazelluläre Vesikel (EVs), die von Erythrozyten bei der Apoptose und bei Einwirken verschiedener Stressoren gebildet werden. Bei der Prozessierung und Lagerung von EKs akkumulieren RMPs in unphysiologischer Menge, und möglicherweise sind diese RMPs anders als jene, die in vivo gebildet werden. Ob RMPs direkte Effekte auf Malignomzellen haben, wurde noch nicht untersucht.
Das Forschungsgebiet rund um EVs ist relativ jung, weshalb noch keine echten Goldstandards bei Isolierung und Quantifizierung vorliegen. Während bei den RMPs hierfür am häufigsten Ultrazentrifugation (UZ) und Durchflusszytometrie verwendet werden, haben beide Methoden gewisse Einschränkungen. Mit der Größenausschlusschromatographie (size exclusion chromatography, SEC) liegt ein Verfahren vor, das sich bei anderen EVs als effektive Alternative zur UZ gezeigt hat und das zudem die Eigenschaften und biologischen Aktivitäten der empfindlichen EVs möglicherweise besser erhält.
Ziel dieser Arbeit war es, im Zellkulturmodell zu untersuchen, ob RMPs aus EKs möglicherweise einen Einfluss auf Viabilität, Migration und Invasion maligner Zellen haben. Hierzu wurde die Kolonkarzinomzelllinie HCT-116 genutzt. Zudem sollte mit der SEC eine alternative Isolierungsmethode für RMPs etabliert werden und ein möglicher Einfluss der Isolierungsmethode auf die biologische Aktivität der RMPs untersucht werden.
Insgesamt zeigte sich in den in vitro-Untersuchungen ein geringer Effekt von RMPs auf die Viabilität, Migration und Invasion von HCT-116-Zellen und dies auch nur in sehr hohen Konzentrationen, die in der Hämotherapie eines Patienten vermutlich nie erreicht werden. Es gilt, diese Beobachtungen in weiterführenden in vivo-Studien (zum Beispiel in Tiermodellen) zu verifizieren.
Die SEC zeigte sich als gut geeignet zur Isolierung von RMPs im Hinblick auf die RMP-Ausbeute und die Auftrennung der RMPs von Proteinen. Die RMPs, die via SEC isoliert wurden, hatten im Gegensatz zu RMPs, die via UZ isoliert wurden, keinen Einfluss auf die Viabilität von HCT-116-Zellen.
Die primäre Quantifizierungsmethode für RMPs war die Durchflusszytometrie, welche bei der Untersuchung kleiner EVs einige Einschränkungen hat, da die Auflösungsgrenze im Bereich der EV-Größe liegt. Ein Vergleich mit einer für EVs ausgelegten Technik, der Nanopartikel-Tracking-Analyse (NTA), zeigte, dass der Großteil der in den RMP-Isolaten enthaltenen Partikel in der Durchflusszytometrie nicht erkannt wird. Dieses Ergebnis könnte durch eine mangelhafte Sensitivität der Durchflusszytometrie, aber auch durch die Unspezifität der NTA erklärt werden. Es wurde in der NTA keine Färbung verwendet, daher konnten auch andere EVs und Partikel wie Lipoproteine mitgezählt werden.
Komplexe biologische Phänotypen resultieren aus einem koordinierten Zusammenspiel von einer Vielzahl von Genen. Um zu verstehen, wie Krankheiten durch genetische Dysfunktionen
entstehen können, ist es unabdingbar die genetischen Interaktionsnetzwerke in menschlichen Zellen zu entschlüsseln. Eine Identifizierung von Kontext-abhängigen genetischen Interaktionen kann bedeutende Erkenntnisse über die Beziehung von Phänotyp und Genotyp liefern und erklären, wie synergistische Gen-Funktionen die Entstehung von komplexen Krankheiten bedingen.
Gepoolte, kombinatorische CRISPR (kurz für: clustered regularly interspaced short palindromic repeats) Screens stellen eine wirkungsvolle Methode zur simultanen Untersuchung potentieller Interaktionen von einer großen Anzahl von Genen dar. Mit sogenannten multiplex CRISPR
gRNA Bibliotheken werden im Rahmen großangelegter Screens vielzählige kombinatorische Gen-Knockouts in Zellen generiert. Diese multiplex CRISPR gRNA Bibliotheken können aus bis zu hunderttausenden Plasmiden bestehen, die jeweils für eine andere gRNA-Kombination kodieren und auf ein spezifisches Gen-Paar abzielen. Im Gegensatz zu CRISPR Screens für Einzel-Knockouts gehen multiplex CRISPR Screens zur Identifizierung von genetischen Interaktionen mit zusätzlichen Herausforderungen einher: Zum einen wächst der verbundene Arbeitsaufwand für die Konstruktion der multiplex CRISPR gRNA Bibliotheken proportional mit der Anzahl der gewünschten Ziel-Gene, welche die Diversität der Bibliothek bestimmt. In einer idealen gRNA-Bibliothek wären alle gRNA-Sequenzen gleich häufig vorhanden. Jedoch weisen
gRNA-Bibliotheken aufgrund von technischen Beschränkungen gRNA-Sequenzen mit höherer, beziehungsweise niedriger Abundanz auf. Konventionelle Methoden zur Herstellung von
gRNA-Bibliotheken basieren beispielsweise auf iterativen, gepoolten Klonierungsschritten mit PCR-amplifizierten Oligonucleotiden, welche zu einer Ungleichverteilung oder zum Verlust von gRNA-Sequenzen führen können. Daher bieten Methoden zur gRNA-Bibliotheken-Generierung Optimierungspotenzial. Da die Reproduzierbarkeit der Screen-Ergebnisse durch die sogenannte Screening Coverage sichergestellt werden muss, erfordert eine Erhöhung der
Bibliotheks-Diversität gleichzeitig auch eine Vergrößerung des Versuchsmaßstabs und ist mit umfangreichem Zellkultur-Arbeitsaufwand verbunden. Die Screening Coverage gibt die
durchschnittliche Abundanz der einzelnen gRNA-Sequenzen in der Zellpopulation während des Screens an. Aktuelle Richtlinien empfehlen eine Screening Coverage, die zwischen dem 200- bis 1000-fachen Wert der Bibliotheks-Diversität liegt, allerdings fehlen bisher genaue Angaben die auf die verwendete gRNA Bibliothek abgestimmt sind. Deshalb stellt die benötigte Screening Coverage bisher einen limitierenden Faktor dar, der die Anzahl der möglichen Ziel-Gene-Kombinationen in einem Screen beschränkt.
In der vorliegenden Arbeit stellen wir eine neue Methode zur Generierung von multiplex gRNA Bibliotheken mit hohen Diversitäten vor. Die Methode, genannt 3Cs (covalently-closed circular-synthesized) Multiplexing, umgeht iterative, gepoolte Klonierugsschritte mit Restriktionsenzymen und PCR-Amplifikation von gRNA-kodierenden Oligonucleotiden. Wir
zeigen, dass 3Cs Multiplexing auf robuste Weise zur Herstellung von gleichmäßig verteilten multiplex gRNA Bibliotheken verwendet werden kann. Der Verteilungs-Skew, auch Skew-Ratio oder Bibliotheksbreite genannt, ist ein Maß zur Ermittlung der Gleichverteilung der gRNA-Sequenzen in der Bibliothek. Wir zeigen, dass 3Cs multiplex Bibliotheken typischerweise einen Verteilungs-Skew von 2.5 aufweisen, was unter den üblichen Werten von Einzel-gRNA Bibliotheken liegt.
Wir nahmen an, dass die gRNA-Bibliotheksverteilung die Robustheit von gepoolten CRISPR Screens beeinflussen könne und deshalb bei der Auswahl einer geeigneten Screening
Coverage berücksichtigt werden müsse. Um den Einfluss der gRNA-Bibliotheksverteilung auf die Screen-Qualität in Abhängigkeit von der verwendeten Screening Coverage zu untersuchen, generierten wir zwei künstlich fehlverteilte multiplex gRNA-Bibliotheken. Diese wurden, zusätzlich zu einer nahezu gleichverteilten multiplex gRNA-Bibliothek, jeweils mit einer 20- und 200-fachen Screening Coverage in einem kombinatorischen Proliferationsscreen angewandt.
Dadurch konnten wir die gRNA-Bibliotheksverteilung als den bestimmenden Parameter für die benötigte Screening Coverage identifizieren. Zusätzlich konnten wir zeigen, dass 3Cs multiplex gRNA-Bibliotheken auf Grund ihrer gleichmäßigen Verteilung mit minimierter Screening Coverage eingesetzt werden können, was zu einer 10-fachen Reduktion des assoziierten Arbeitsaufwands führt. Während bisherige Richtlinien für gepoolte CRISPR Screens die initiale
gRNA-Bibliotheksverteilung nicht berücksichtigen, empfehlen wir die Screening Coverage an dieser auszurichten.
Autophagie ist ein streng regulierter zellulärer Prozess, der den Lysosomen Abbau von intrazellulärem Material steuert und im Zusammenhang mit zahlreichen menschlichen Erkrankungen steht. Da Autophagie in eine Vielzahl von Signalwegen integriert ist, bietet es außerdem therapeutische Ansatzpunkte zur Behandlung von Krankheiten. Die Identifizierung von synergistischen Funktionen zwischen Autophagie-Genen könnte unser Verständnis über die molekularen Mechanismen, die der Regulation der Autophagie zu Grunde liegen, erweitern und dadurch neuartige Behandlungen ermöglichen.
Um genetische Interaktionen von Autophagie-Genen zu untersuchen haben wir eine 3Cs multiplex gRNA Bibliothek generiert, die auf menschliche Autophagie-Genkombinationen
abzielt. In dieser Arbeit demonstrieren wir die Funktionalität der 3Cs Autophagie multiplex gRNA Bibliothek unter Anwendung minimierter Screening Coverage in zwei verschiedenen Screen-Ausführungen: In einem Proliferationsscreen konnten wir Geninteraktionen
identifizieren, deren Verlust zu einer gesteigerten oder verringerten Zellproliferation führt. Unter diesen resultierte der Knockout von WDR45B-PIK3R4 zur stärksten Suppression der Proliferation, während die Depletion von ATG7-KEAP1 zu extrem verstärkter Proliferation beitrug. Unter Einsatz eines Autophagie-Reporters konnten wir in einem Autophagie Screen genetische Interaktionen aufdecken, die essentiell für Autophagie sind, darunter die
Interaktionen zwischen ATG2A-ATG2B , GABARAPL2-WIPI2 und ULK4-SQSTM1.
Wir glauben, dass 3Cs Multiplexing in Zukunft breite Anwendung in verschiedenen biologisch relevanten Feldern finden kann und die Entschlüsselung von kontext-abhängigen genetischen Interaktionen voranbringen und so das Verständnis für die Entstehung von komplexen pathologischen Phänotypen erweitern wird.
NOSTRIN belongs to the family of F-BAR proteins, which are multi-domain adaptor proteins that have emerged as important regulators of membrane remodeling and actin dynamics in a variety of vital cellular processes. They have been analyzed structurally and biochemically and overexpression studies have revealed their potential in inducing membrane curvature and tubulation. Several studies have begun to decipher the function of individual proteins, but the understanding of F-BAR protein functions in vivo is still quite limited. The F-BAR protein NOSTRIN is mainly expressed in endothelial cells and has originally been described as interaction partner of the endothelial nitric oxide synthase (eNOS), modulating eNOS subcellular localization. The phenotypic characterization of NOSTRIN knockout mice revealed decreased nitric oxide (NO) and cGMP levels, an increase in systolic blood pressure and an impairment of the acetylcholine-induced, NO-dependent relaxation of aortic rings from mice with global as well as endothelial cell-specific knockout of the NOSTRIN gene (ECKO) . These findings implied that NOSTRIN plays a role in regulating NO production in vivo, but the underlying molecular mechanisms were unclear. Therefore, this study was aimed at addressing the mechanism causing the inhibited vasodilation specifically upon stimulation with acetylcholine in NOSTRIN KO and ECKO mice, and at exploring additional roles of NOSTRIN in the signal transduction of endothelial cells.
The major acetylcholine receptor that mediates vessel relaxation upon stimulation with acetylcholine is the muscarinic acetylcholine receptor subtype M3 (M3R). In the present study NOSTRIN was identified as novel interaction partner of the M3R and important factor for the correct spatial distribution and functionality of the M3R. Moreover, it provides the first example of an F-BAR protein regulating a GPCR. Confocal immunofluorescence microscopy analysis of isolated aortae from NOSTRIN KO and WT mice indicated that NOSTRIN was necessary for the proper subcellular localization of the M3R and targeted it to the plasma membrane. A series of pulldown experiments revealed a direct interaction of NOSTRIN with the M3R. The binding required the SH3 domain of NOSTRIN and the third intracellular loop of the M3R, which has a recognized role in receptor regulation. The interaction of NOSTRIN with the M3R was confirmed by co-localization of NOSTRIN and the M3R upon overexpression in mammalian cells. Expression levels of the M3R as well as eNOS were not affected by the loss of NOSTRIN in accordance with the finding, that NOSTRIN impacts on the acetylcholine/eNOS signaling axis through regulation of the subcellular trafficking of its binding partners.
Furthermore, there were first indications for a role of NOSTRIN in facilitating the carbachol-induced calcium response in M3R-expressing cells, suggesting that NOSTRIN might influence M3R activation. in the absence of NOSTRIN, the function of the M3R in mammalian cells overexpressing the M3R was markedly impaired, resulting in abolition of the calcium response to the M3R agonist carbachol. In accordance, the activated eNOS fraction associated with the Golgi complex was markedly reduced in aorta explants from NOSTRIN knockout and ECKO mice. Moreover, NOSTRIN knockout inhibited the carbachol-induced, activating phosphorylation of eNOS in murine aortae as well as primary mouse lung endothelial cells confirming its role as important regulator of eNOS activity in vivo.
Ubiquitylation is a three-step process, which results in the attachment of the small protein ubiquitin (Ub) to lysine residues on a substrate protein. SUMO proteins are ubiquitin (Ub)-related modifiers implicated in the regulation of gene transcription, cell cycle, DNA repair and protein localization. The molecular mechanisms by which the sumoylation of target proteins regulates diverse cellular functions remain poorly understood. During my PhD I isolated and characterized SUMO1 and SUMO2 binding motifs. Using Yeast Two Hybrid system, bioinformatics and NMR spectroscopy we defined a common SUMO-interacting motif (SIM) and map its binding surfaces on SUMO1 and SUMO2. This motif forms a β-strand that could bind in parallel or anti-parallel orientation to the β2-strand of SUMO due to the environment of the hydrophobic core. A negative charge imposed by a stretch of neighboring acidic amino acids and/or phosphorylated serine residues determines its specificity in binding to distinct SUMO paralogues and can modulate the spatial orientation of SUMO-SIM interactions. Mutation of the SUMO interacting motif of TTRAP (TRAFS and TNF receptor associated protein) influences both its localization and dynamic behaviour in living cells. Ubiquitin (Ub)-binding domains (UBDs) are key elements in conveying Ub-based cellular signals. UBD-containing proteins interact with ubiquitylated targets and control numerous biological processes including receptor trafficking, DNA repair, virus budding and gene transcription. They themselves undergo UBD-dependent monoubiquitylation, which promotes intramolecular binding of the UBD to the attached Ub and consequently leads to their functional inhibition. During the second part of my PhD I could show that, in contrast to the established ubiquitylation pathway, the presence of UBDs allows the monoubiquitylation of host protein independently of classical E3 ligases. UBDs of different types including UBA, UIM, UBM, NFZ and UBZ, can directly cooperate with E2 Ub-conjugating enzymes to promote monoubiquitylation of their host proteins. Using FRET technology I verified that the E2 enzyme and the substrate directly interact in cells. Moreover, UBD-containing proteins Stam2 and Sts2 promote self-ubiquitylation and not ubiquitylation of other targets or form polyUb chains from free Ub. Our study revealed a yet unappreciated role of E2 enzymes in ubiquitylation reactions of UBD containing proteins.
Die Fähigkeit der spezifischen und kontextabhängigen zellulären Adaption auf intrinsische und/oder extrinsische Signale ist das Fundament zellulärer Homöostase. Verschiedene Signale werden von Membranrezeptoren oder intrazellulären Rezeptoren erkannt und ermöglichen die molekulare Anpassung zellulärer Prozesse. Komplexe, ineinandergreifende Proteinnetzwerke sind dabei elementar in der Regulation der Zelle. Proteine und deren Funktionen werden dabei nach Bedarf reguliert und unterliegen einem ständigen proteolytischen Umsatz.
Die stimulusabhängige Gentranskription und/oder Proteintranslation nimmt hier eine zentrale Stellung ein, da die zugrundeliegende Maschinerie die Komposition und Funktion der Proteinnetzwerke entsprechend anpassen kann. Zusätzlich zur Regulation der Proteinabundanz werden Proteine posttranslational modifiziert, um deren Eigenschaften rasch zu ändern. Zu posttranslationalen Modifikationen zählen die Ubiquitinierung und/oder Phosphorylierung, welche die Proteinfunktionen hochdynamisch regulieren. Deregulierte Proteinnetzwerke werden oft mit Neurodegeneration und Autoimmun- oder Krebserkrankungen assoziiert. Auch Infektionen mit humanpathogenen Bakterien greifen stark in den Regulierungsprozess von Proteinnetzwerken und deren Funktionen ein. Die zelluläre Homöostase wird dadurch herausgefordert.
Bakterien der Gattung Salmonella sind zoonotische, gramnegative, fakultativ intrazelluläre Pathogene, welche weltweit millionenfach Salmonellen-erkrankungen hervorrufen. Von besonderer Bedeutung ist dabei Salmonella enterica serovar Typhimurium (hiernach Salmonella), welches im Menschen, meist durch mangelnde Hygienemaßnahmen, Gastroenteritis auslöst.
Immunität in Epithelzellen wird über das angeborene Immunsystem vermittelt und dient der Pathogenerkennung und -bekämpfung. Die Toll-like Rezeptoren (TLR) gehören zu den Mustererkennungsrezeptoren (pattern recognition receptors), welche spezifische mikrobielle Strukturen detektieren und eine kontextabhängige zelluläre Antwort generieren. Danger-Rezeptoren erkennen hingegen nicht direkt das Pathogen, sondern zelluläre Perturbationen, welche durch Zellschäden oder bakterielle Invasionen verursacht werden. Die intrinsische Fähigkeit der Wirtszelle, sich gegen Infektionen/Gefahren zu wehren wird dabei als zellautonome Immunität bezeichnet. Dabei nehmen induzierte proinflammatorische Signalwege und zelluläre Stressantworten eine wichtige Stellung ein. Die zelluläre Stressantwort aktiviert unter anderem die selektive Autophagie. Diese kann spezifisch aberrante Organelle, Proteine und invasive Pathogene abbauen. Ein weiterer Stresssignalweg ist die integrated stress response (ISR), welche eine selektive Proteintranslation erlaubt und damit die Auflösung des proteintoxischen Stresses ermöglicht.
Zur Penetration von Epithelzellen benötigt Salmonella ein komplexes System an Virulenzfaktoren, welches die bakterielle Internalisierung und Proliferation in der Wirtszelle ermöglicht. Salmonella nutzt dazu ein Typ-III-Sekretionssystem. Das System sekretiert bakterielle Virulenzfaktoren in die Zelle, sodass eine hochspezifische Modulierung des Wirtes erzwungen wird.
Die Virulenzfaktoren SopE und SopE2 spielen dabei eine Schlüsselrolle, da sie die Pathogenität von Salmonella maßgeblich vermitteln. Durch molekulare Mimikry von Wirts GTP (Guanosintriphosphat) -Austauschfaktoren aktivieren SopE und SopE2 die Rho GTPasen CDC42 und Rac1. GTP-geladenes CDC42 und Rac1 wiederum aktivieren das Aktinzytoskelett und stimulieren die Polymerisierung von Aktinfilamenten über den Arp2/3-Komplex an der Invasionsstelle. Das Pathogen wird dadurch in ein membranumhülltes Vesikel, die sogenannte Salmonella-containing Vakuole (SCV), aufgenommen. Die SCV stellt eine protektive, replikative, intrazelluläre Nische des Pathogens dar und wird permanent durch verschiedene Virulenzfaktoren moduliert.
Im Allgemeinen führt die Aktivierung von Mustererkennungsrezeptoren und Danger-Rezeptoren also zu einer zellulären Stressantwort und Entzündungsreaktion, wodurch es zur Bekämpfung der Infektion kommt. Inflammatorische Signalwege werden meist über den zentralen Transkriptionsfaktor NF-κB (nuclear factor 'kappa-light-chain-enhancer' of activated B-cells) vermittelt. NF-κB bewirkt die Induktion von proinflammatorischen Effektoren und Stressgenen. Zellautonome Immunität wird zusätzlich durch antibakterielle Autophagie ermöglicht, wobei Salmonella selektiv über das lysosomale System abgebaut werden. Das bakterielle Typ-III-Sekretionssystem verursacht an einigen wenigen SCVs Membranschäden, sodass Salmonella das Wirtszytosol penetrieren. Zytosolische Bakterien werden dabei spezifisch ubiquitiniert. Dies erlaubt die Erkennung durch die Autophagie-Maschinerie.
In der vorliegenden Arbeit wurde die zellautonome Immunität von Epithelzellen während einer akuten Salmonella Infektion durch quantitative Proteomik untersucht...
Lysosomes are major degradative organelles that contain enzymes capable of breaking down proteins, nucleic acids, carbohydrates, and lipids. In the last decade, new discoveries have traced also important roles for lysosomes as signalling hubs, affecting metabolism, autophagy and pathogenic infections. Therefore, maintenance of a healthy lysosome population is of utmost importance to the cell to respond to both stress conditions and also homeostatic signalling. For example, for minor perturbations to the lysosomal membrane, the cell activates repair processes which seal membrane nicks. For more extensive damage, autophagy is activated to remove damaged organelles from the cell. on the other hand, during pathogen invasion host cells have also evolved mechanisms to hijack the endolysosomal pathway to facilitate their own growth and replication in host cells.
The first part of the thesis work focuses on a lysosomal regeneration program which is activated under conditions where the entire lysosomal pool of the cell is damaged. Upon extensive membrane damage induced by the lysosomotropic drug LLOMe, the cell activates a regeneration pathway which helps in the formation of new functional lysosomes by recycling damaged membranes. I have identified the molecules important for this novel pathway of lysosomal regeneration and showed how the protein TBC1D15 orchestrates this process to regenerate functional organelles from completely damaged membrane masses in the first 2 hours following lysosomal membrane damage. This process resembles the process of auto- lysosomal reformation (ALR)- involving the formation of lysosomal tubules which are extended along microtubules and cleaved in a dynamin2 dependent manner to form proto-lysosomes which develop into fully functional mature lysosomes. These lysosomal tubules are closely associated with ATG8 positive autophagosomal membranes and require ATG8 proteins to bind to the lysophagy receptor LIMP2 on damaged membranes. This process is physiologically important under conditions of crystal nephropathy where calcium oxalate crystals induce damage to lysosomal membranes in nephrons in kidney disease.
The second part of the thesis shows how the endolysosomal system of the cell is hijacked by the bacteriaLegionella pneumophila. During Legionella infection the formation of conventional ATG8 positive autophagosomes are blocked due to the protease activity of the bacterial effector protein RavZ which cleaves lipidated ATG8 proteins from autophagosomal membranes. The SidE effectors of Legionella modify STX17 and SNAP29 by the process of non-canonical ubiquitination called phosphoribose-linked serine ubiquitination (PR-Ub). These proteins are essential for the formation of the autophagosomal SNARE complex which is used for fusion of the autophagosome with the lysosome. Upon Legionella infection, PR-UB of STX17 aids in formation of autophagosome-like replication vacuoles. ThesevacuolesdonotfusewiththelysosomebecauseSNAP29isalsoPR-Ubmodified. PR-UbofSTX17 and SNAP29 sterically blocks the formation of the autophagosomal-SNARE complex thereby preventing fusion of the autophagosome with the lysosome. As a result, Legionella can replicate in autophagosome- like vacuoles which do not undergo lysosomal degradation. In absence of PR-Ub modified STX17, bacterial replication is compromised when measured by bacterial replication assays in lung epithelial (A549) cells.
Taken together, this thesis highlights two important aspects of the autophagy-lysosomal system- how it responds to extensive membrane damage and its importance in Legionella pneumophila infection. Extensive damage to lysosomal membranes triggers a rapid regeneration process to partially restore lysosomal function before the effects of TFEB dependent lysosomal biogenesis becomes apparent. On the other hand, Legionella pneumophila infection segregates the lysosomes from the rest of the endo-lysosomal system by blocking autophagosome-lysosome fusion. Though lysosomes remain active, they are incapable of degrading pathogens since pathogen containing vacuoles do not fuse with the lysosome.