TY  - THES
A1  - Zimmermann, Henriette
T1  - Antigenic variation and stumpy development in \(Trypanosoma\)  \(brucei\)
T1  - Antigene Variation und Stumpy Entwicklung in \(Trypanosoma\)  \(brucei\)
N2  - The eukaryotic parasite Trypanosoma brucei has evolved sophisticated strategies to persist within its mammalian host. Trypanosomes evade the hosts' immune system by antigenic variation of their surface coat, consisting of variant surface glycoproteins (VSGs). Out of a repertoire of thousands of VSG genes, only one is expressed at any given time from one of the 15 telomeric expression sites (ES). The VSG is stochastically exchanged either by a transcriptional switch of the active ES (in situ switch) or by a recombinational exchange of the VSG within the active ES. However, for infections to persist, the parasite burden has to be limited. The slender (sl) bloodstream form secretes the stumpy induction factor (SIF), which accumulates with rising parasitemia. SIF induces the irreversible developmental transition from the proliferative sl to the cell cycle-arrested but fly-infective stumpy (st) stage once a concentration threshold is reached. Thus, antigenic variation and st development ensure persistent infections and transmissibility. A previous study in monomorphic cells indicated that the attenuation of the active ES could be relevant for the development of trypanosomes. The present thesis investigated this hypothesis using the inducible overexpression of an ectopic VSG in pleomorphic trypanosomes, which possess full developmental competence. These studies revealed a surprising phenotypic plasticity: while the endogenous VSG was always down-regulated upon induction, the ESactivity determined whether the VSG overexpressors arrested in growth or kept proliferating. Full ES-attenuation induced the differentiation of bona fide st parasites independent of the cell density and thus represents the sole natural SIF-independent differentiation trigger to date. A milder decrease of the ES-activity did not induce phenotypic changes, but appeared to prime the parasites for SIF-induced differentiation. These results demonstrate that antigenic variation and development are linked and indicated that the ES and the VSG are independently regulated. Therefore, I investigated in the second part of my thesis how ES-attenuation and VSG-silencing can be mediated. Integration of reporters with a functional or defective VSG 3'UTR into different genomic loci showed that the maintenance of the active state of the ES depends on a conserved motif within the VSG 3'UTR. In situ switching was only triggered when the telomere-proximal motif was partially deleted, suggesting that it serves as a DNA-binding motif for a telomere-associated protein. The VSG levels seem to be additionally regulated in trans based on the VSG 3'UTR independent of the genomic context, which was reinforced by the regulation of a constitutively expressed reporter with VSG 3' UTR upon ectopic VSG overexpression.
N2  - Der eukaryotische Parasit Trypanosoma brucei hat komplexe Strategien entwickelt, um in seinem Säugetierwirt zu überleben. Die Grundlage der Immunevasion ist die antigene Variation des Oberflächenmantels, der aus dem variablen Oberflächenglykoprotein (VSG) besteht. Von mehreren tausend VSG-Genen wird zu jedem Zeitpunkt nur ein einziges aus einer der 15 telomerischen Expressionsstellen (ES) exprimiert. Das VSG kann entweder durch einen transkriptionellen Wechsel der aktiven ES (in situ Wechsel) oder durch einen rekombinatorischen Wechsel des VSG-Gens innerhalb der aktiven ES stochastisch ausgetauscht werden. Damit jedoch eine langanhaltende Infektion des Wirts möglich wird, muss gleichzeitig der Parasitenbefall begrenzt werden. Mit ansteigender Parasitämie akkumuliert der 'stumpy induction factor' (SIF), welcher von der 'slender' (sl) Blutstromform sekretiert wird. Sobald ein Schwellenwert in der SIF-Konzentration erreicht ist, wird die irreversible Differenzierung der proliferativen sl in die zellzyklusarretierte 'stumpy'(st) Form eingeleitet, welche infektiös für den Fliegenvektor ist. Somit stellen antigene Variation und st- Differenzierung das Persistieren der Infektion und die Übertragung des Parasiten sicher. Eine frühere Arbeit mit monomorphen Zellen deutete darauf hin, dass die Attenuierung der aktiven ES eine Rolle für die Differenzierung der Trypanosomen spielen könnte. Diese Hypothese wurde in der vorliegenden Dissertation untersucht, indem in pleomorphen Zellen mit vollständiger Entwicklungskompetenz ein ektopisches VSG induzierbar überexprimiert wurde. Diese Studien offenbarten eine erstaunliche phänotypische Plastizität: während das endogene VSG nach Induktion runter reguliert wurde, arretierten die VSG-Überexpressoren in Abhängigkeit von der ES-Aktivität entweder im Wachstum oder teilten sich weiter. Die vollständige ES-Attenuierung löste die Differenzierung zu echten st Zellen unabhängig von der Zelldichte aus und ist somit der bisher einzige natürliche SIF-unabhängige Differenzierungsauslöser. Eine mildere Abnahme der ES-Aktivität verursachte keinen Phänotyp, scheint aber die Zellen auf die SIF-induzierte Differenzierung vorzubereiten. Diese Ergebnisse zeigen, dass antigene Variation und Differenzierung verbunden sind und deuteten an, dass die ES und das VSG unabhängig voneinander reguliert werden. Daher habe ich im zweiten Teil meiner Dissertation untersucht, wie ES-Attenuierung und VSG-Stilllegung vermittelt werden können. Die Integration eines Reporters mit funktioneller oder defekter VSG 3'UTR an verschiedenen Orten im Genom zeigte, dass die Aufrechterhaltung der ES-Aktivität von einem konservierten Motiv in der VSG 3'UTR abhängig ist. Ein in situ Wechsel wurde nur ausgelöst, wenn Teile des Telomer-proximalen Motiv deletiert wurden, was nahelegt, dass das Motiv auf DNA-Ebene von einem Telomerbindeprotein erkannt wird. Die VSG-Level scheinen unabhängig vom genomischen Kontext zusätzlich in trans basierend auf der VSG 3'UTR reguliert zu werden, was durch die Regulation eines konstitutiv exprimierten Reporters mit VSG 3'UTR nach VSG-Überexpression bekräftigt wurde.
KW  - Trypanosoma brucei
KW  - Genexpression
KW  - Entwicklung
KW  - Parasit
KW  - VSG
KW  - antigenic variation
KW  - monoallelic expression
KW  - stumpy development
KW  - differentiation
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-146902
ER  - 
TY  - JOUR
A1  - Schuster, Sarah
A1  - Lisack, Jaime
A1  - Subota, Ines
A1  - Zimmermann, Henriette
A1  - Reuter, Christian
A1  - Mueller, Tobias
A1  - Morriswood, Brooke
A1  - Engstler, Markus
T1  - Unexpected plasiticty in the life cycle of Trypanosoma brucei
JF  - eLife
N2  - African trypanosomes cause sleeping sickness in humans and nagana in cattle. These unicellular parasites are transmitted by the bloodsucking tsetse fly. In the mammalian host’s circulation, proliferating slender stage cells differentiate into cell cycle-arrested stumpy stage cells when they reach high population densities. This stage transition is thought to fulfil two main functions: first, it auto-regulates the parasite load in the host; second, the stumpy stage is regarded as the only stage capable of successful vector transmission. Here, we show that proliferating slender stage trypanosomes express the mRNA and protein of a known stumpy stage marker, complete the complex life cycle in the fly as successfully as the stumpy stage, and require only a single parasite for productive infection. These findings suggest a reassessment of the traditional view of the trypanosome life cycle. They may also provide a solution to a long-lasting paradox, namely the successful transmission of parasites in chronic infections, despite low parasitemia.
KW  - trypanosoma
KW  - sleeping sickness
KW  - tsetse fly
KW  - transmission
KW  - life cycle
KW  - development
Y1  - 2021
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-261744
VL  - 10
ER  - 
TY  - JOUR
A1  - Zimmermann, Henriette
A1  - Subota, Ines
A1  - Batram, Christopher
A1  - Kramer, Susanne
A1  - Janzen, Christian J.
A1  - Jones, Nicola G.
A1  - Engstler, Markus
T1  - A quorum sensing-independent path to stumpy development in Trypanosoma brucei
JF  - PLoS Pathogens
N2  - For persistent infections of the mammalian host, African trypanosomes limit their population size by quorum sensing of the parasite-excreted stumpy induction factor (SIF), which induces development to the tsetse-infective stumpy stage. We found that besides this cell density-dependent mechanism, there exists a second path to the stumpy stage that is linked to antigenic variation, the main instrument of parasite virulence. The expression of a second variant surface glycoprotein (VSG) leads to transcriptional attenuation of the VSG expression site (ES) and immediate development to tsetse fly infective stumpy parasites. This path is independent of SIF and solely controlled by the transcriptional status of the ES. In pleomorphic trypanosomes varying degrees of ES-attenuation result in phenotypic plasticity. While full ES-attenuation causes irreversible stumpy development, milder attenuation may open a time window for rescuing an unsuccessful antigenic switch, a scenario that so far has not been considered as important for parasite survival.
KW  - Trypanosoma
KW  - hyperexpression techniques
KW  - parasitic cell cycles
KW  - cloning
KW  - cell cycle and cell division
KW  - cell differentiation
KW  - tetracyclines
KW  - parasitic diseases
Y1  - 2017
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-158230
VL  - 13
IS  - 4
ER  - 
TY  - JOUR
A1  - El-Helou, Sabine M.
A1  - Biegner, Anika-Kerstin
A1  - Bode, Sebastian
A1  - Ehl, Stephan R.
A1  - Heeg, Maximilian
A1  - Maccari, Maria E.
A1  - Ritterbusch, Henrike
A1  - Speckmann, Carsten
A1  - Rusch, Stephan
A1  - Scheible, Raphael
A1  - Warnatz, Klaus
A1  - Atschekzei, Faranaz
A1  - Beider, Renata
A1  - Ernst, Diana
A1  - Gerschmann, Stev
A1  - Jablonka, Alexandra
A1  - Mielke, Gudrun
A1  - Schmidt, Reinhold E.
A1  - Schürmann, Gesine
A1  - Sogkas, Georgios
A1  - Baumann, Ulrich H.
A1  - Klemann, Christian
A1  - Viemann, Dorothee
A1  - Bernuth, Horst von
A1  - Krüger, Renate
A1  - Hanitsch, Leif G.
A1  - Scheibenbogen, Carmen M.
A1  - Wittke, Kirsten
A1  - Albert, Michael H.
A1  - Eichinger, Anna
A1  - Hauck, Fabian
A1  - Klein, Christoph
A1  - Rack-Hoch, Anita
A1  - Sollinger, Franz M.
A1  - Avila, Anne
A1  - Borte, Michael
A1  - Borte, Stephan
A1  - Fasshauer, Maria
A1  - Hauenherm, Anja
A1  - Kellner, Nils
A1  - Müller, Anna H.
A1  - Ülzen, Anett
A1  - Bader, Peter
A1  - Bakhtiar, Shahrzad
A1  - Lee, Jae-Yun
A1  - Heß, Ursula
A1  - Schubert, Ralf
A1  - Wölke, Sandra
A1  - Zielen, Stefan
A1  - Ghosh, Sujal
A1  - Laws, Hans-Juergen
A1  - Neubert, Jennifer
A1  - Oommen, Prasad T.
A1  - Hönig, Manfred
A1  - Schulz, Ansgar
A1  - Steinmann, Sandra
A1  - Klaus, Schwarz
A1  - Dückers, Gregor
A1  - Lamers, Beate
A1  - Langemeyer, Vanessa
A1  - Niehues, Tim
A1  - Shai, Sonu
A1  - Graf, Dagmar
A1  - Müglich, Carmen
A1  - Schmalzing, Marc T.
A1  - Schwaneck, Eva C.
A1  - Tony, Hans-Peter
A1  - Dirks, Johannes
A1  - Haase, Gabriele
A1  - Liese, Johannes G.
A1  - Morbach, Henner
A1  - Foell, Dirk
A1  - Hellige, Antje
A1  - Wittkowski, Helmut
A1  - Masjosthusmann, Katja
A1  - Mohr, Michael
A1  - Geberzahn, Linda
A1  - Hedrich, Christian M.
A1  - Müller, Christiane
A1  - Rösen-Wolff, Angela
A1  - Roesler, Joachim
A1  - Zimmermann, Antje
A1  - Behrends, Uta
A1  - Rieber, Nikolaus
A1  - Schauer, Uwe
A1  - Handgretinger, Rupert
A1  - Holzer, Ursula
A1  - Henes, Jörg
A1  - Kanz, Lothar
A1  - Boesecke, Christoph
A1  - Rockstroh, Jürgen K.
A1  - Schwarze-Zander, Carolynne
A1  - Wasmuth, Jan-Christian
A1  - Dilloo, Dagmar
A1  - Hülsmann, Brigitte
A1  - Schönberger, Stefan
A1  - Schreiber, Stefan
A1  - Zeuner, Rainald
A1  - Ankermann, Tobias
A1  - Bismarck, Philipp von
A1  - Huppertz, Hans-Iko
A1  - Kaiser-Labusch, Petra
A1  - Greil, Johann
A1  - Jakoby, Donate
A1  - Kulozik, Andreas E.
A1  - Metzler, Markus
A1  - Naumann-Bartsch, Nora
A1  - Sobik, Bettina
A1  - Graf, Norbert
A1  - Heine, Sabine
A1  - Kobbe, Robin
A1  - Lehmberg, Kai
A1  - Müller, Ingo
A1  - Herrmann, Friedrich
A1  - Horneff, Gerd
A1  - Klein, Ariane
A1  - Peitz, Joachim
A1  - Schmidt, Nadine
A1  - Bielack, Stefan
A1  - Groß-Wieltsch, Ute
A1  - Classen, Carl F.
A1  - Klasen, Jessica
A1  - Deutz, Peter
A1  - Kamitz, Dirk
A1  - Lassy, Lisa
A1  - Tenbrock, Klaus
A1  - Wagner, Norbert
A1  - Bernbeck, Benedikt
A1  - Brummel, Bastian
A1  - Lara-Villacanas, Eusebia
A1  - Münstermann, Esther
A1  - Schneider, Dominik T.
A1  - Tietsch, Nadine
A1  - Westkemper, Marco
A1  - Weiß, Michael
A1  - Kramm, Christof
A1  - Kühnle, Ingrid
A1  - Kullmann, Silke
A1  - Girschick, Hermann
A1  - Specker, Christof
A1  - Vinnemeier-Laubenthal, Elisabeth
A1  - Haenicke, Henriette
A1  - Schulz, Claudia
A1  - Schweigerer, Lothar
A1  - Müller, Thomas G.
A1  - Stiefel, Martina
A1  - Belohradsky, Bernd H.
A1  - Soetedjo, Veronika
A1  - Kindle, Gerhard
A1  - Grimbacher, Bodo
T1  - The German national registry of primary immunodeficiencies (2012-2017)
JF  - Frontiers in Immunology
N2  - Introduction: The German PID-NET registry was founded in 2009, serving as the first national registry of patients with primary immunodeficiencies (PID) in Germany. It is part of the European Society for Immunodeficiencies (ESID) registry. The primary purpose of the registry is to gather data on the epidemiology, diagnostic delay, diagnosis, and treatment of PIDs. 

Methods: Clinical and laboratory data was collected from 2,453 patients from 36 German PID centres in an online registry. Data was analysed with the software Stata® and Excel. 

Results: The minimum prevalence of PID in Germany is 2.72 per 100,000 inhabitants. Among patients aged 1-25, there was a clear predominance of males. The median age of living patients ranged between 7 and 40 years, depending on the respective PID. Predominantly antibody disorders were the most prevalent group with 57% of all 2,453 PID patients (including 728 CVID patients). A gene defect was identified in 36% of patients. Familial cases were observed in 21% of patients. The age of onset for presenting symptoms ranged from birth to late adulthood (range 0-88 years). Presenting symptoms comprised infections (74%) and immune dysregulation (22%). Ninety-three patients were diagnosed without prior clinical symptoms. Regarding the general and clinical diagnostic delay, no PID had undergone a slight decrease within the last decade. However, both, SCID and hyper IgE-syndrome showed a substantial improvement in shortening the time between onset of symptoms and genetic diagnosis. Regarding treatment, 49% of all patients received immunoglobulin G (IgG) substitution (70%-subcutaneous; 29%-intravenous; 1%-unknown). Three-hundred patients underwent at least one hematopoietic stem cell transplantation (HSCT). Five patients had gene therapy. 

Conclusion: The German PID-NET registry is a precious tool for physicians, researchers, the pharmaceutical industry, politicians, and ultimately the patients, for whom the outcomes will eventually lead to a more timely diagnosis and better treatment.
KW  - registry for primary immunodeficiency
KW  - primary immunodeficiency (PID)
KW  - German PID-NET registry
KW  - PID prevalence
KW  - European Society for Immunodeficiencies (ESID)
KW  - IgG substitution therapy
KW  - CVID
Y1  - 2019
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-226629
VL  - 10
ER  -