Vera Catherine Hirschfeld-Warneken
Max Planck Society
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Featured researches published by Vera Catherine Hirschfeld-Warneken.
Nano Letters | 2008
Marco Arnold; Vera Catherine Hirschfeld-Warneken; Theobald Lohmüller; Patrick Heil; Jacques Blümmel; Elisabetta Ada Cavalcanti-Adam; Mónica López-García; Paul Walther; Horst Kessler; Benjamin Geiger; Joachim P. Spatz
Cell interactions with adhesive surfaces play a vital role in the regulation of cell proliferation, viability, and differentiation, and affect multiple biological processes. Since cell adhesion depends mainly on the nature and density of the adhesive ligand molecules, spatial molecular patterning, which enables the modulation of adhesion receptor clustering, might affect both the structural and the signaling activities of the adhesive interaction. We herein show that cells plated on surfaces that present a molecularly defined spacing gradient of an integrin RGD ligand can sense small but consistent differences in adhesive ligand spacing of about 1 nm across the cell diameter, which is approximately 61 mum when the spacing includes 70 nm. Consequently, these positional cues induce cell polarization and initiate cell migration and signaling. We propose that differential positional clustering of the integrin transmembrane receptors is used by cells for exploring and interpreting their environment, at high spatial sensitivity.
The Journal of Neuroscience | 2008
M. A. Willaredt; Kerstin Hasenpusch-Theil; H. A. R. Gardner; I. Kitanovic; Vera Catherine Hirschfeld-Warneken; C. P. Gojak; K. Gorgas; C. L. Bradford; Joachim P. Spatz; Stefan Wölfl; Thomas Theil; Kerry Lee Tucker
Primary cilia are important sites of signal transduction involved in a wide range of developmental and postnatal functions. Proteolytic processing of the transcription factor Gli3, for example, occurs in primary cilia, and defects in intraflagellar transport (IFT), which is crucial for the maintenance of primary cilia, can lead to severe developmental defects and diseases. Here we report an essential role of primary cilia in forebrain development. Uncovered by N-ethyl-N-nitrosourea-mutagenesis, cobblestone is a hypomorphic allele of the IFT gene Ift88, in which Ift88 mRNA and protein levels are reduced by 70–80%. cobblestone mutants are distinguished by subpial heterotopias in the forebrain. Mutants show both severe defects in the formation of dorsomedial telencephalic structures, such as the choroid plexus, cortical hem and hippocampus, and also a relaxation of both dorsal-ventral and rostral-caudal compartmental boundaries. These defects phenocopy many of the abnormalities seen in the Gli3 mutant forebrain, and we show that Gli3 proteolytic processing is reduced, leading to an accumulation of the full-length activator isoform. In addition, we observe an upregulation of canonical Wnt signaling in the neocortex and in the caudal forebrain. Interestingly, the ultrastructure and morphology of ventricular cilia in the cobblestone mutants remains intact. Together, these results indicate a critical role for ciliary function in the developing forebrain.
Hfsp Journal | 2008
Elisabetta Ada Cavalcanti-Adam; Daniel Aydin; Vera Catherine Hirschfeld-Warneken; Joachim P. Spatz
During adhesion and spreading, cells form micrometer‐sized structures comprising transmembrane and intracellular protein clusters, giving rise to the formation of what is known as focal adhesions. Over the past two decades these structures have been extensively studied to elucidate their organization, assembly, and molecular composition, as well as to determine their functional role. Synthetic materials decorated with biological molecules, such as adhesive peptides, are widely used to induce specific cellular responses dependent on cell adhesion. Here, we focus on how surface patterning of such bioactive materials and organization at the nanoscale level has proven to be a useful strategy for mimicking both physical and chemical cues present in the extracellular space controlling cell adhesion and fate. This strategy for designing synthetic cellular environments makes use of the observation that most cell signaling events are initiated through recruitment and clustering of transmembrane receptors by extracellular‐presented signaling molecules. These systems allow for studying protein clustering in cells and characterizing the signaling response induced by, e.g., integrin activation. We review the findings about the regulation of cell adhesion and focal adhesion assembly by micro‐ and nanopatterns and discuss the possible use of substrate stiffness and patterning in mimicking both physical and chemical cues of the extracellular space.
European Journal of Cell Biology | 2008
Vera Catherine Hirschfeld-Warneken; Marco Arnold; Ada Cavalcanti-Adam; Mónica López-García; Horst Kessler; Joachim P. Spatz
In vivo cell migration and location are orchestrally guided by soluble and bound chemical gradients. Here, gradients of extracellular matrix molecules are formed synthetically by the combination of a surface nanopatterning technique called block copolymer nanolithography (BCN) and a biofunctionalisation technique. A modified substrate dip-coating process of BCN allows for the formation of precise molecular gradients of cyclic RGDfK peptide patches at interfaces, which are presented to cells for testing cell adhesion and polarisation. Surfaces formed by BCN consist of hexagonally ordered gold dot patterns with a gradient in particle spacing. Each dot serves as a chemical anchor for the binding of cyclic RGDfK peptides, which are specifically recognised by alpha(v)beta(3) integrins. Due to steric hindrance only up to one integrin binds to one functionalised gold dot which forms a peptide patch spacing. We demonstrate how cell morphology, adhesion area, actin and vinculin distribution as well as cell body polarisation are influenced by the peptide patch spacing gradient. As a consequence, these gradients of adhesive ligands induce cell orientation towards smaller particle spacing when the gradient strength is 15nm/mm at least. This implicates that an adherent cells sensitivity to differentiate between ligand patch spacing is approximately 1nm across the cell body.
Journal of Cell Science | 2013
Nadav Elad; Tova Volberg; Israel Patla; Vera Catherine Hirschfeld-Warneken; Carsten Grashoff; Joachim P. Spatz; Reinhard Fässler; Benjamin Geiger; Ohad Medalia
Summary Integrin-mediated focal adhesions (FAs) are large, multi-protein complexes that link the actin cytoskeleton to the extracellular matrix and take part in adhesion-mediated signaling. These adhesions are highly complex and diverse at the molecular level; thus, assigning particular structural or signaling functions to specific components is highly challenging. Here, we combined functional, structural and biophysical approaches to assess the role of a major FA component, namely, integrin-linked kinase (ILK), in adhesion formation. We show here that ILK plays a key role in the formation of focal complexes, early forms of integrin adhesions, and confirm its involvement in the assembly of fibronectin-bound fibrillar adhesions. Examination of ILK-null fibroblasts by cryo-electron tomography pointed to major structural changes in their FAs, manifested as disarray of the associated actin filaments and an increase in the packing density of FA-related particles. Interestingly, adhesion of the mutant cells to the substrate required a higher ligand density than in control cells. These data indicate that ILK has a key role in integrin adhesion assembly and sub-structure, and in the regulation of the FA-associated cytoskeleton.
Nano Letters | 2013
Katharina Klein; Timo Maier; Vera Catherine Hirschfeld-Warneken; Joachim P. Spatz
Phenotyping of tumor cells by marker-free quantification is important for cancer diagnostics. For the first time, fractal analysis of reflection interference contrast microscopy images of single living cells was employed as a new method to distinguish between different nanoscopic membrane features of tumor cells. Since tumor progression correlates with a higher degree of chaos within the cell, it can be quantified mathematically by fractality. Our results show a high accuracy in identifying malignant cells with a failure chance of 3%, which is far better than today’s applied methods.
Biointerphases | 2013
Katharina Klein; Christina Rommel; Vera Catherine Hirschfeld-Warneken; Joachim P. Spatz
Reflection interference contrast microscopy (RICM) allows the visualization of the cell’s adhesion topology on substrates. Here it is applied as a new label-free method to measure adhesion forces between tumor cells and their substrate without any external manipulation, i.e., the application of force or adjustments in the substrate elasticity. Malignant cancer transformation is closely associated with the down-regulation of adhesion proteins and the consequent reduction of adhesion forces. By analyzing the size and distribution of adhesion patches from a benign and a malignant human pancreatic tumor cell line, we established a model for calculating the adhesion strength based on RICM images. Further, we could show that the cell’s spread area does not necessarily scale with adhesion strength. Despite the larger projected cell area of the malignant cell line, adhesion strength was clearly reduced. This underscores the importance of adhesion patch analysis. The calculated force values were verified by microfluidic detachment assays. Static and dynamic RICM measurements produce numerous adhesion-related parameters from which characteristic cell signatures can be derived. Such a cellular fingerprint can refine the process of categorizing cell lines according to their grade of differentiation.
International Journal of Materials Research | 2011
Daniel Aydin; Vera Catherine Hirschfeld-Warneken; Ilia Louban; Joachim P. Spatz
Abstract Intelligent interfaces make use of a fundamental molecular understanding of biosystems for the induction of their specific responses. Biological cells especially have an enormous spatial resolution for organizing their transmembrane receptor molecules, which is translated into specific cell functions. In turn, interfaces which provide a counter organization of molecules to required transmembrane receptor organizations are able to induce specific cell responses accordingly. This mission requires a patterning technology at interfaces which operates at the resolution of single molecules. Here, we report on self-assembly technologies for providing such patterns and their subsequent functionalization with cell receptor binding molecules. Cells explore such surfaces and show a very distinct cell response. In the future, such interfaces may “learn” how to induce cell responses properly by analyzing cell responses and providing dynamically the adequate interface pattern which will allow cells to act more...
Nature Cell Biology | 2010
Israel Patla; Tova Volberg; Nadav Elad; Vera Catherine Hirschfeld-Warneken; Carsten Grashoff; Reinhard Fässler; Joachim P. Spatz; Benjamin Geiger; Ohad Medalia
Intelligent Surfaces in Biotechnology: Scientific and Engineering Concepts, Enabling Technologies, and Translation to Bio-Oriented Applications | 2012
Daniel Aydin; Vera Catherine Hirschfeld-Warneken; Ilia Louban; Joachim P. Spatz