Search

Your search keyword '"Martin Lensch"' showing total 26 results
Start Over Author "Martin Lensch"
26 results on '"Martin Lensch"'

1. Toward Comprehensive Analysis of the Galectin Network in Chicken: Unique Diversity of Galectin-3 and Comparison of its Localization Profile in Organs of Adult Animals to the Other Four Members of this Lectin Family

Author

Wolf D. Lehmann, Dolores Solís, Sabine André, Joachim C. Manning, Michaela Lohr, Martin Lensch, Joerg Seidler, Hans-Joachim Gabius, Dieter Kübler, Lara López-Merino, Herbert Kaltner, Ministerio de Ciencia e Innovación (España), and Centro de Investigación Biomédica en Red Enfermedades Respiratorias (España)

Subjects
Histology, Galectin 3, Blotting, Western, Molecular Sequence Data, Computational biology, Biology, Epithelium, Immunoenzyme Techniques, Transcription (biology), Animals, Humans, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Phosphorylation, Promoter Regions, Genetic, Gene, Peptide sequence, Phylogeny, Ecology, Evolution, Behavior and Systematics, Glycoproteins, Galectin, Genetics, Messenger RNA, Reverse Transcriptase Polymerase Chain Reaction, Macrophages, Gene Expression Profiling, Alternative splicing, Promoter region, Promoter, Gene expression profiling, Alternative Splicing, Anatomy, Lectin, Chickens, Biotechnology
Abstract

18 pags, 11 figs, 2 tabs. -- Additional Supporting Information may be found in the online version of this article, Characterization of all members of a gene family established by gene divergence is essential to delineate distinct or overlapping expression profiles and functionalities. Their activity as potent modulators of diverse physiological processes directs interest to galectins (endogenous lectins with β-sandwich fold binding β-galactosides and peptide motifs), warranting their study with the long-term aim of a comprehensive analysis. The comparatively low level of complexity of the galectin network in chicken with five members explains the choice of this organism as model. Previously, the three proto-type chicken galectins CG-1A, CG-1B, and CG-2 as well as the tandem-repeat-type CG-8 had been analyzed. Our study fills the remaining gap to determine gene structure, protein characteristics and expression profile of the fifth protein, that is, chimera-type chicken galectin-3 (CG-3). Its gene has a unique potential to generate variants: mRNA production stems from two promoters, alternative splicing of the form from the second transcription start point (tsp) can generate three mRNAs. The protein with functional phosphorylation sites in the N-terminus generated by transcription from the first tsp (tsp1CG-3) is the predominant CG-3 type present in adult tissues. Binding assays with neoglycoproteins and cultured cells disclose marked similarity to properties of human galectin-3. The expression and localization profiles as well as proximal promoter regions have characteristic features distinct from the other four CGs. This information on CG-3 completes the description of the panel of CGs, hereby setting the stage for detailed comparative analysis of the entire CG family, e.g., in embryogenesis. © 2011 Wiley-Liss, Inc., Spanish Ministry of Science and Innovation Grant number: BFU2009-10052; Grant sponsor: CIBER of Respiratory Diseases (CIBERES) (ISCII)

Published
2011

2. Analysis of MonoPEGylated Human Galectin-2 by Small-Angle X-ray and Neutron Scattering: Concentration Dependence of PEG Conformation in the Conjugate

Author

Martin Lensch, Vasil M Garamus, Conan J. Fee, Tracey Hanley, Hans-Joachim Gabius, Lizhong He, Anton P. J. Middelberg, and Hui Wang

Subjects
Polymers and Plastics, Galectin 2, Protein Stability, Small-angle X-ray scattering, Chemistry, X-Rays, Molecular Conformation, Concentration effect, Bioengineering, Polyethylene glycol, Small-angle neutron scattering, Polyethylene Glycols, Biomaterials, Neutron Diffraction, chemistry.chemical_compound, Crystallography, Solubility, Scattering, Small Angle, PEG ratio, Materials Chemistry, PEGylation, Radius of gyration, Humans, Conjugate
Abstract

Protein conjugation with polyethylene glycol (PEG) is a valuable means for improving stability, solubility, and bioavailability of pharmaceutical proteins. Using human galectin-2 (hGal-2) and 5 kDa PEG as a model system we first produced a PEG-hGal-2 conjugate exclusively at the Cys75 residue, resulting in two monosubstituted subunits per hGal-2 homodimer. Small angle X-ray and neutron scattering (SAXS and SANS) were combined to provide complementary structural information about the PEG-hGal-2 conjugate, wherein signal generation in SAXS depends mainly on the protein while SANS data presents signals from both the protein and PEG moieties. SAXS data gave a constant radius of gyration (R(g) = 21.5 Å) for the conjugate at different concentrations and provided no evidence for an alteration of homodimeric structure or hGal-2 ellipsoidal shape upon PEGylation. In contrast, SANS data revealed a concentration dependence of R(g) for the conjugate, with the value decreasing from 31.5 Å at 2 mg/mL to 26 Å at 14 mg/mL (based on hGal-2 concentration). Scattering data have been successfully described by the model of the ellipsoidal homogeneous core (hGal-2) attached with polymer chains (PEG) at the surface. Evidently, the PEG conformation of the conjugate strongly depends on conjugate concentration and PEG's radius of gyration decreases from 24.5 to 15 Å. An excluded volume effect, arising from steric clashes between PEG molecules at high concentration, was quantified by estimating the second virial coefficient, A(2), of PEGylated hGal-2 from the SANS data. A positive value of A(2) (6.0 ± 0.4 × 10(-4) cm(3) mol g(-2)) indicates repulsive interactions between molecules, which are expected to protect the PEGylated protein against aggregation.

Published
2010

3. Carbamate-Linked Lactose: Design of Clusters and Evidence for Selectivity to Block Binding of Human Lectins to (Neo)Glycoproteins with Increasing Degree of Branching and to Tumor Cells

Author

Valentin Wittmann, Nicolai V. Bovin, Martin Lensch, Daniel Specker, Herbert Kaltner, Sabine André, and Hans-Joachim Gabius

Subjects
Glycan, Carbamate, medicine.medical_treatment, Drug Evaluation, Preclinical, Biomedical Engineering, Pharmaceutical Science, Lactose, Bioengineering, Plasma protein binding, Branching (polymer chemistry), chemistry.chemical_compound, Lectins, Neoplasms, medicine, Humans, Glycoproteins, Pharmacology, chemistry.chemical_classification, biology, Chemistry, Organic Chemistry, Lectin, carbohydrates (lipids), Biochemistry, Drug Design, ddc:540, biology.protein, Carbamates, Selectivity, Glycoprotein, Protein Binding, Biotechnology
Abstract

Various pathogenic processes are driven by protein(lectin)-glycan interactions, especially involving beta-galactosides at branch ends of cellular glycans. These emerging insights fuel the interest to design potent inhibitors to block lectins. As a step toward this aim, we prepared a series of ten mono- to tetravalent glycocompounds with lactose as a common headgroup. To obtain activated carbonate for ensuing carbamate formation, conditions for the facile synthesis of pure isomers from anomerically unprotected lactose were identified. To probe for the often encountered intrafamily diversity of human lectins, we selected representative members from the three subgroups of adhesion/growth-regulatory galectins as receptors. Diversity of the glycan display was accounted for by using four (neo)glycoproteins with different degrees of glycan branching as matrices in solid-phase assays. Cases of increased inhibitory potency of lactose clusters compared to free lactose were revealed. Extent of relative inhibition was not directly associated with valency in the glycocompound and depended on the lectin type. Of note for screening protocols, efficacy of blocking appeared to decrease with increased degree of glycan branching in matrix glycoproteins. Binding to tumor cells was impaired with selectivity for galectins-3 and -4. Representative compounds did not impair growth of carcinoma cells up to a concentration of 5 mM of lactose moieties (valence-corrected value) per assay. The reported bioactivity and the delineation of its modulation by structural parameters of lectins and glycans set instructive examples for the further design of selective inhibitors and assay procedures.

Published
2009

4. Single-Site Cys-Substituting Mutation of Human Lectin Galectin-2: Modulating Solubility in Recombinant Production, Reducing Long-Term Aggregation, and Enabling Site-Specific MonoPEGylation

Author

Anton P. J. Middelberg, Lizhong He, Hans-Joachim Gabius, Martin Lensch, Conan J. Fee, and Hui Wang

Subjects
Polymers and Plastics, Galectin 2, Protein Conformation, Protein subunit, Bioengineering, medicine.disease_cause, Polyethylene Glycols, law.invention, Biomaterials, law, Lectins, Materials Chemistry, medicine, Humans, Cysteine, Protein secondary structure, Galectin, chemistry.chemical_classification, Mutation, biology, Protein Stability, Effector, Lectin, Recombinant Proteins, Amino Acid Substitution, Solubility, chemistry, Biochemistry, Mutagenesis, Site-Directed, biology.protein, Recombinant DNA, Glycoprotein, Dimerization
Abstract

The effector capacity of endogenous lectins on cell adhesion/growth prompts studies to turn them into pharmaceutically stable forms. Using human galectin-2 as a proof-of-principle model, we first introduced mutations at the site of one of the two Cys residues, that is, C57A, C57M, and C57S. Only the C57M variant was expressed in bacteria in soluble form in high yield. No notable aggregation of the modified homodimeric lectin occurred during 3 weeks of storage. This mutational process also facilitated the site-directed introduction of poly(ethylene glycol) into the remaining sulfhydryl group (Cys75). Product analysis revealed rather complete conjugation with one chain per subunit in the homodimer. We note that neither the secondary structure alteration nor the absence of binding ability to a glycoprotein (asialofetuin) was observed. The results thus document the feasibility of tailoring a human galectin for enhanced stability to aggregation as well as monoPEGylation, which enables further testing of biological properties including functionality as growth regulator and the rate of serum clearance.

Published
2008

5. Cell-type-specific expression of murine multifunctional galectin-3 and its association with follicular atresia/luteolysis in contrast to pro-apoptotic galectins-1 and -7

Author

Sabine André, Fred Sinowatz, Herbert Kaltner, Martin Lensch, Hans-Joachim Gabius, and Michaela Lohr

Subjects
endocrine system, medicine.medical_specialty, Histology, Galectin 1, Galectin 3, Galectins, Granulosa cell, Follicular Atresia, Luteolysis, Apoptosis, Biology, Mice, Internal medicine, otorhinolaryngologic diseases, medicine, Animals, Promoter Regions, Genetic, Zona pellucida, Molecular Biology, Galectin, Mice, Knockout, urogenital system, Follicular atresia, Computational Biology, Cell Biology, Immunohistochemistry, Cell biology, Mice, Inbred C57BL, Medical Laboratory Technology, medicine.anatomical_structure, Endocrinology, Organ Specificity, Galectin-3, Galectin-1, DNA fragmentation, Female
Abstract

Galectin-3 is a multifunctional protein with modular design. A distinct expression profile was determined in various murine organs when set into relation to homodimeric galectins-1 and -7. Fittingly, the signature of putative transcription-factor-binding sites in the promoter region of the galectin-3 gene affords a toolbox for a complex combinatorial regulation, distinct from the respective sequence stretches in galectins-1 and -7. A striking example for cell-type specificity was the ovary, where these two lectins were confined to the surface epithelium. Immunohistochemically, galectin-3 was found in macrophages of the cortical interstitium between developing follicles and medullary interstitium, matching the distribution of the F4/80 antigen. With respect to atresia and luteolysis strong signals in granulosa cells of atretic preantral but not antral follicles and increasing positivity in corpora lutea upon regression coincided with DNA fragmentation. Labeled galectin-3 revealed lactose-inhibitable binding to granulosa cells. Also, slender processes of vital granulosa cells which extended into the zona pellucida were positive. This study demonstrates cell-type specificity and cycle-associated regulation for galectin-3 with increased presence in atretic preantral follicles and in late stages of luteolysis.

Published
2008

6. Human galectins as sensors for apoptosis/necrosis-associated surface changes of granulocytes and lymphocytes

Author

Herbert Kaltner, Martin Herrmann, Peter Kern, Alexandra Beer, Connie Schulze, Hans-Joachim Gabius, Kerstin Sarter, Sabine André, Udo S. Gaipl, Martin Lensch, and Sandra Franz

Subjects
Programmed cell death, Histology, Necrosis, Galectins, Cell, Apoptosis, Biology, Pathology and Forensic Medicine, Flow cytometry, chemistry.chemical_compound, Annexin, otorhinolaryngologic diseases, medicine, Humans, Lymphocytes, Propidium iodide, Galectin, Cell Death, medicine.diagnostic_test, Cell Biology, Flow Cytometry, Cell biology, medicine.anatomical_structure, chemistry, medicine.symptom, Granulocytes
Abstract

Changes in the glycomic profile can significantly affect the cells' communication with the environment. Plant lectins have so far been used to address the issue as to whether the courses of apoptosis or necrosis are associated with such alterations. We, here, initiate the study of members of the family of functionally pleiotropic human galectins in this respect. Established protocols for the induction of apoptosis/necrosis of blood cells and for flow cytometry using annexin V/propidium iodide were combined with cell surface staining using biotinylated galectins at a nontoxic concentration. The galectin panel covered members from all three subfamilies. Flow cytometry revealed specific binding of galectins to viable control cells and conspicuous staining differences when testing apoptotic or necrotic cells. Onset and especially progression of cell death led to pronounced reactivity with the proto-type galectins-1, -2, and -7 and tandem-repeat-type galectin-4. Extent of staining depended on the nature and stage of cell death, type of dying cell, and type of galectin. Galectins act as sensors for cell-death-associated surface changes. Staining of late-apoptotic polymorphonuclear cells was particularly strong. Examining the functional significance of this result may reveal a new aspect within the surveillance system to protect against autoinflammation. © 2008 International Society for Analytical Cytology

Published
2008

7. Prototype chicken galectins revisited: characterization of a third protein with distinctive hydrodynamic behaviour and expression pattern in organs of adult animals

Author

Michaela Lohr, Martina Schnölzer, Jürgen Kopitz, Herbert Kaltner, Martin Lensch, José L. Saiz, Michael Mürnseer, Joachim C. Manning, Sabine André, Hans-Joachim Gabius, and Dolores Solís

Subjects
Prototype chicken galectin, animal structures, Galectins, Molecular Sequence Data, Biology, Biochemistry, Homology (biology), Avian Proteins, Protein structure, Species Specificity, Nephron, Gene duplication, Animals, Amino Acid Sequence, Cloning, Molecular, Binding site, Protein Structure, Quaternary, Molecular Biology, Peptide sequence, Phylogeny, Galectin, Binding Sites, Gene Expression Profiling, Promoter region, Lectin, Cell Biology, Molecular biology, Homology, Cell biology, Gene expression profiling, biology.protein, Chickens
Abstract

Prototype galectins are versatile modulators of cell adhesion and growth via their reactivity to certain carbohydrate and protein ligands. These functions and the galectins' marked developmental regulation explain their attractiveness as models to dissect divergent evolution after gene duplication. Only two members have so far been assumed to constitute this group in chicken, namely the embryonic muscle/liver form {C-16 or CLL-I [16 kDa; chicken lactose lectin, later named CG-16 (chicken galectin-16)]} and the embryonic skin/intestine form (CLL-II or C-14; later named CG-14). In the present study, we report on the cloning and expression of a third prototype CG. It has deceptively similar electrophoretic mobility compared with recombinant C-14, the protein first isolated from embryonic skin, and turned out to be identical with the intestinal protein. Hydrodynamic properties unusual for a homodimeric galectin and characteristic traits in the proximal promoter region set it apart from the two already known CGs. Their structural vicinity to galectin-1 prompts their classification as CG-1A (CG-16)/CG-1B (CG-14), whereas sequence similarity to mammalian galectin-2 gives reason to refer to the intestinal protein as CG-2. The expression profiling by immunohistochemistry with specific antibodies discerned non-overlapping expression patterns for the three CGs in several organs of adult animals. Overall, the results reveal a network of three prototype galectins in chicken.

Published
2007

8. Gene-expression signature of adhesion/growth-regulatory tissue lectins (galectins) in transitional cell cancer and its prognostic relevance

Author

Hans-Joachim Gabius, P. Alken, M. Hatzinger, Specht K, Martin Lensch, Sigrun Langbein, Sabine André, Jasmin Katrin Badawi, Herbert Kaltner, Brinck U, Brade J, and Urology

Subjects
Pathology, medicine.medical_specialty, Histology, animal structures, Galectins, Gene Expression, Pathology and Forensic Medicine, Gene expression, medicine, otorhinolaryngologic diseases, Humans, Urothelium, Cell adhesion, Galectin, Neoplasm Staging, Carcinoma, Transitional Cell, Binding Sites, biology, Reverse Transcriptase Polymerase Chain Reaction, Lectin, Cancer, General Medicine, medicine.disease, Prognosis, DNA Fingerprinting, Immunohistochemistry, stomatognathic diseases, Urinary Bladder Neoplasms, Cell culture, Cancer research, biology.protein
Abstract

Aims: Lectins, and especially galectins, appear to be important in malignancy-associated processes. The aim was to analyse comprehensively the presence of galectins in urothelial tumours. Methods and results: Non-cross-reactive antibodies against seven family members from the three subgroups (prototype: galectin-1, -2 and -7; chimera type: galectin-3; tandem-repeat type: galectin-4, -8 and -9) were used. Gene expression was monitored in specimens of normal urothelium, fresh tumour tissue and cell lines by real-time polymerase chain reaction (PCR). The presence and evidence of tumour-associated up-regulation were shown for galectin-1 and -3. This was less clear-cut for galectin-4 and -8. Galectin-7 was expressed in all cell lines; galectin-2 and -9 were detected at comparatively low levels. Galectin-2, -3 and -8 up-regulation was observed in superficial tumours, but not in muscle-invasive tumours (P

Published
2007

9. Interaction profile of galectin-5 with free saccharides and mammalian glycoproteins: probing its fine specificity and the effect of naturally clustered ligand presentation

Author

Albert M. Wu, Tanuja Singh, Sabine André, Hans-Joachim Gabius, Martin Lensch, and June H. Wu

Subjects
Glycan, Glycosylation, Glycoconjugate, Galectins, Molecular Sequence Data, Oligosaccharides, Enzyme-Linked Immunosorbent Assay, Plasma protein binding, Biochemistry, chemistry.chemical_compound, Animals, Humans, Amino Acid Sequence, Peptide sequence, Glycoproteins, Galectin, chemistry.chemical_classification, biology, Rats, Carbohydrate Sequence, chemistry, Docking (molecular), biology.protein, Glycoprotein, Protein Binding
Abstract

Cell-surface glycans are functional docking sites for tissue lectins such as the members of the galectin family. This interaction triggers a wide variety of responses; hence, there is a keen interest in defining its structural features. Toward this aim, we have used enzyme-linked lectinosorbent (ELLSA) and inhibition assays with the prototype rat galectin-5 and panels of free saccharides and glycoconjugates. Among 45 natural glycans tested for lectin binding, galectin-5 reacted best with glycoproteins (gps) presenting a high density of Galbeta1-3/4GlcNAc (I/II) and multiantennary N-glycans with II termini. Their reactivities, on a nanogram basis, were up to 4.3 x 10(2), 3.2 x 10(2), 2.5 x 10(2), and 1.7 x 10(4) times higher than monomeric Galbeta1-3/4GlcNAc (I/II), triantennary-II (Tri-II), and Gal, respectively. Galectin-5 also bound well to several blood group type B (Galalpha1-3Gal)- and A (GalNAcalpha1-3Gal)-containing gps. It reacted weakly or not at all with tumor-associated Tn (GalNAcalpha1-Ser/Thr) and sialylated gps. Among the mono-, di-, and oligosaccharides and mammalian glycoconjugates tested, blood group B-active II (Galalpha1-3Gal beta1-4GlcNAc), B-active IIbeta1-3L (Galalpha1-3Galbeta1-4GlcNAc beta1-3Galbeta1-4Glc), and Tri-II were the best. It is concluded that (1) Galbeta1-3/4GlcNAc and other Galbeta1-related oligosaccharides with alpha1-3 extensions are essential for binding, their polyvalent form in cellular glycoconjugates being a key recognition force for galectin-5; (2) the combining site of galectin-5 appears to be of a shallow-groove type sufficiently large to accommodate a substituted beta-galactoside, especially with alpha-anomeric extension at the non-reducing end (e.g., human blood group B-active II and B-active IIbeta1-3L); (3) the preference within beta-anomeric positioning is Galbeta1-4 > or = Galbeta1-3 > Galbeta1-6; and (4) hydrophobic interactions in the vicinity of the core galactose unit can enhance binding. These results are important for the systematic comparison of ligand selection in this family of adhesion/growth-regulatory effectors with potential for medical applications.

Published
2006

10. Unique sequence and expression profiles of rat galectins-5 and -9 as a result of species-specific gene divergence

Author

Hans-Joachim Gabius, Martin Lensch, Michaela Lohr, Sabine André, Roland Russwurm, Herbert Kaltner, and Michel Vidal

Subjects
animal structures, Galectins, Molecular Sequence Data, Biology, Biochemistry, Mice, Gene duplication, otorhinolaryngologic diseases, Animals, Erythropoiesis, Tissue Distribution, Amino Acid Sequence, RNA, Messenger, Promoter Regions, Genetic, Gene, Peptide sequence, Galectin, Regulation of gene expression, Base Sequence, Epidermis (botany), Gene Expression Profiling, Chromosome Mapping, Genetic Variation, Cell Biology, Immunohistochemistry, Rats, Gene expression profiling, stomatognathic diseases, Gene Expression Regulation
Abstract

Presence of species-specific gene divergence in a protein family prompts to thoroughly study structural aspects and expression profiles of the products. We herein focus on two members of an adhesion/growth-regulatory group of endogenous lectins, i.e. galectins-5 and -9. After first ascertaining species specificity of occurrence of galectin-5, constituted by a short section of rat galectin-9's N-terminal part and its C-terminal carbohydrate recognition domain, by database mining, we next detected and defined sequence differences in the proximal promoter region between the two genes. The ensuing hypothesis for distinct expression profiles was tested first by RT-PCR and then by immunohistochemistry. For the latter purpose, we employed antibodies rigorously controlled for absence of cross-reactivity including assays with various other galectins and, if necessary, refined by chromatographic removal of bi- or oligospecific activities. Indeed, the galectins have non-identical expression profiles, qualitative differences, e.g. seen for galectin-5-positive bone marrow and erythrocytes or for hitherto unknown expression in cells of the theca folliculi and galectin-9-positive skin epidermis and esophageal epithelium. Lack of hepatocyte or renal cortex staining separates these two expression profiles in rat from localization of galectin-9 in mouse. Interspecies extrapolation in a case of a galectin involved in unique gene divergence may thus not be valid. The presented results on galectin-5 relative to galectin-9 intimate distinct functions especially in erythropoiesis and imply currently unknown mechanisms to compensate its absence from the galectin network in other mammals.

Published
2006

11. Introduction of extended LEC14-type branching into core-fucosylated biantennary N-glycan

Author

Ingo Prahl, Sabine André, Hans-Joachim Gabius, Shuji Kojima, Martin Lensch, and Carlo Unverzagt

Subjects
chemistry.chemical_classification, Biodistribution, Glycan, Glycosylation, biology, Lectin, Mannose, Cell Biology, Oligosaccharide, Biochemistry, Epitope, chemistry.chemical_compound, chemistry, biology.protein, Molecular Biology, Galectin
Abstract

A series of enzymatic substitutions modifies the basic structure of complex-type biantennary N-glycans. Among them, a β1,2-linked N-acetylglucosamine residue is introduced to the central mannose moiety of the core-fucosylated oligosaccharide by N-acetylglucosaminyltransferase VII. This so-called LEC14 epitope can undergo galactosylation at the β1,2-linked N-acetylglucosamine residue. Guided by the hypothesis that structural modifications in the N-glycan alter its capacity to serve as ligand for lectins, we prepared a neoglycoprotein with the extended LEC14 N-glycan and tested its properties in three different assays. In order to allow comparison to previous results on other types of biantennary N-glycans the functionalization of the glycans for coupling and assay conditions were deliberately kept constant. Compared to the core-fucosylated N-glycan no significant change in affinity was seen when testing three galactoside-specific proteins. However, cell positivity in flow cytofluorimetry was enhanced in six of eight human tumor lines. Analysis of biodistribution in tumor-bearing mice revealed an increase of blood clearance by about 40%, yielding a favorable tumor/blood ratio. Thus, the extended LEC14 motif affects binding properties to cellular lectins on cell surfaces and organs when compared to the core-fucosylated biantennary N-glycan. The results argue in favor of the concept of viewing substitutions as molecular switches for lectin-binding affinity. Moreover, they have potential relevance for glycoengineering of reagents in tumor imaging.

Published
2005

12. Human Galectin-2: Novel Inducer of T Cell Apoptosis with Distinct Profile of Caspase Activation

Author

Axel Dignass, Sabine André, Martin Lensch, Hans-Joachim Gabius, Herbert Kaltner, Stefan Rosewicz, Bertram Wiedenmann, and Andreas Sturm

Subjects
CD3 Complex, Galectin 1, Galectin 2, Galectins, T-Lymphocytes, Immunology, Integrin, Cell, Apoptosis, Antigens, CD7, Lymphocyte Activation, Membrane Potentials, Proto-Oncogene Proteins, Sequence Homology, Nucleic Acid, Cell Adhesion, otorhinolaryngologic diseases, medicine, Animals, Humans, Immunology and Allergy, Binding site, bcl-2-Associated X Protein, Galectin, Sequence Homology, Amino Acid, biology, Caspase 3, Effector, Integrin beta1, Cell Cycle, Galactosides, Intracellular Membranes, Cell cycle, Molecular biology, Caspase 9, Mitochondria, Rats, Cell biology, Enzyme Activation, stomatognathic diseases, medicine.anatomical_structure, Proto-Oncogene Proteins c-bcl-2, Caspases, biology.protein, Cytokines, Cytokine secretion, Protein Binding
Abstract

Galectin-2 is structurally closely related to galectin-1, but has a distinct expression profile primarily confined to the gastrointestinal tract. Prominent differences in the proximal promoter regions between galectins-2 and -1 concern Sp1-, hepatocyte NF-3, and T cell-specific factor-1 binding sites. Of note, these sequence elements are positioned equally in the respective regions for human and rat galectins-2. Labeled galectin-2 binds to T cells in a β-galactoside-specific manner. In contrast to galectin-1, the glycoproteins CD3 and CD7 are not ligands, while the shared affinity to β1 integrin (or a closely associated glycoprotein) accounts for a substantial extent of cell surface binding. The carbohydrate-dependent binding of galectin-2 induces apoptosis in activated T cells. Fluorogenic substrate and inhibitor assays reveal involvement of caspases-3 and -9, in accordance with cleavage of the DNA fragmentation factor. Enhanced cytochrome c release, disruption of the mitochondrial membrane potential, and an increase of the Bax/Bcl-2 ratio by opposite regulation of expression of both proteins add to the evidence that the intrinsic apoptotic pathway is triggered. Cell cycle distribution and expression of regulatory proteins remained unaffected. Notably, galectins-1 and -7 reduce cyclin B1 expression, defining functional differences between the structurally closely related galectins. Cytokine secretion of activated T cells was significantly shifted to the Th2 profile. Our study thus classifies galectin-2 as proapoptotic effector for activated T cells, raising a therapeutic perspective. Of importance for understanding the complex galectin network, it teaches the lesson that selection of cell surface ligands, route of signaling, and effects on regulators of cell cycle progression are markedly different between structurally closely related galectins.

Published
2004

13. New aspects of galectin functionality in nuclei of cultured bone marrow stromal and epidermal cells: biotinylated galectins as tool to detect specific binding sites

Author

Jiřá Klíma, Barbora Dvořánková, Corina Böck, Zuzana Holíková, Martin Lensch, Tereza Purkrábková, Karel Smetana, Robert Pytlik, Sabine André, Hans-Joachim Gabius, Fu-Tong Liu, and Jan Motlik

Subjects
Stromal cell, Swine, Galectins, Bone Marrow Cells, Biology, otorhinolaryngologic diseases, medicine, Animals, Humans, Biotinylation, Proliferation Marker, Binding site, Cells, Cultured, Galectin, Cell Nucleus, Fibrillarin, Binding Sites, Cell Biology, General Medicine, Molecular biology, medicine.anatomical_structure, Epidermal Cells, Bone marrow, Epidermis, Stromal Cells, Stem cell
Abstract

Nuclear presence of galectins suggests a role of these endogenous lectins in the regulation of transcription, pre-mRNA splicing and transport processes. Therefore, detection and localization of nuclear binding sites for galectins by a new methodological step, has potential to further functional analysis. In the first step of our model study we monitored the nuclear expression of galectins-1 and -3 in cultured stromal cells of human bone marrow and human/porcine keratinocytes. To enable detection and localization of galectin-specific binding sites, we used purified galectins biotinylated without loss of activity as cytochemical tool. The degree of labeling of the probes was determined by adapting two-dimensional gel electrophoresis and calculating pI changes in response to stepwise chemical modification of basic and acidic side chains by the biotinylation reagents. Binding studies revealed positivity for galectin-1, whereas galectins-3, -5, and -7 were not reactive with nuclear sites under identical conditions in bone marrow stromal cells and keratinocytes prepared from hair follicle enriched for stem cells. Inhibition by lactose indicated an involvement of the carbohydrate recognition domain in nuclear binding of galectin-1. Colocalization of the galectin-1-dependent signal with the SC35 splicing factor and sensitivity toward RNase treatment argued in favor of galectin binding in nuclear speckles, albeit only for a small fraction of the cells. Epidermal cells positive for galectin-1-binding sites expressed DeltaNp63 known as a potential marker of stem cells. Based on cytokeratin expression cells with nuclear binding of labeled galectin-1 were basal and not suprabasal cells. Regarding proliferation, no relationship to the expression of a proliferation marker, Ki-67, was observed. The nucleolar signal colocalized with fibrillarin and nucleophosmin/B23 as representatives of nucleolar proteins in both types of studied cells. In conclusion, the application of labeled galectins to localize accessible binding sites adds a new aspect to the functional analysis of these lectins in the nucleus.

Published
2003

14. Adhesion/growth-regulatory galectins: insights into their ligand selectivity using natural glycoproteins and glycotopes

Author

Albert M, Wu, Tanuja, Singh, Jia-Hau, Liu, Sabine, André, Martin, Lensch, Hans-Christian, Siebert, Mickael, Krzeminski, Alexandre M J J, Bonvin, Herbert, Kaltner, June H, Wu, and Hans-Joachim, Gabius

Subjects
Mammals, Models, Molecular, Binding Sites, Base Sequence, Galectins, Molecular Sequence Data, Galactose, Epithelial Cells, Ligands, Substrate Specificity, Epitopes, Structure-Activity Relationship, Cell Adhesion, Animals, Amino Acid Sequence, Promoter Regions, Genetic, Chickens, Glycoproteins, Protein Binding
Published
2011

15. N-domain of human adhesion/growth-regulatory galectin-9: preference for distinct conformers and non-sialylated N-glycans and detection of ligand-induced structural changes in crystal and solution

Author

Jesús Jiménez-Barbero, Hans-Joachim Gabius, Lara López-Merino, Jürgen Kopitz, João P. Ribeiro, Margarita Menéndez, Michaela Lohr, F. Javier Cañada, Maria J. Maté, Martin Lensch, Sabine André, Antonio A. Romero, José L. Saiz, Herbert Kaltner, Gunter Haroske, Federico M. Ruiz, Matthias Kloor, Dolores Solís, Uwe Wollina, and Eliza Buzamet

Subjects
Circular dichroism, Glycosylation, Stereochemistry, Protein Conformation, Galectins, Disaccharide, Lactose, Plasma protein binding, CHO Cells, Cell Growth Processes, Antiparallel (biochemistry), Crystallography, X-Ray, Ligands, Biochemistry, chemistry.chemical_compound, Protein structure, Cricetulus, Cricetinae, Cell Adhesion, Animals, Humans, Nuclear Magnetic Resonance, Biomolecular, Galectin, Ligand, Protein Stability, Cell Biology, chemistry, Crystallization, Protein Binding
Abstract

Human tandem-repeat-type galectin-9 is a potent adhesion/growth-regulatory effector via lectin capacity of its N- and C-terminal domains. This bioactivity prompted further crystallographic study of the N-domain, combined with analysis in solution. Binding of lactose markedly increased the N-domain's resistance to thermal denaturation. Crystallography revealed its intimate contact profile, besides detecting an extension of the beta-sandwich fold by an antiparallel beta-strand F0 aligned to the C-terminal F1 strand. Ligand accommodation in its low-energy conformation leads to a movement of Arg87's side chain. As consequence, the ligand's glucose moiety and Arg87 become hydrogen bonded. The resulting predictions for spatial parameters in solution were verified by determining (a) the pattern of magnetization transfer from the protein to protons of lactose and Forssman disaccharide by NMR spectroscopy and (b) the ellipticity changes at wavelengths characteristic for Trp/Tyr residues in near-UV CD spectroscopy. Whereas solid-phase assays confirmed a previously noted tendency for homo- and heterotypic aggregation, gel filtration and ultracentrifugation disclosed monomeric status in solution, in line with crystallographic data. Using cell mutants with defects in glycosylation, this lectin domain was shown to preferentially bind N-glycans without alpha2,3-sialylation. Since proximal promoter sequences were delineated to diverge markedly among galectin genes and resulting differences in expression profiles were exemplarily documented immunohistochemically, the intrafamily diversification appears to have assigned this protein to a characteristic expression and activity profile among galectins. Our data thus take the crystallographic information to the level of the lectin in solution and in tissues by a strategic combination of spectroscopic and cell/histochemical assays.

Published
2009

16. Unique chicken tandem-repeat-type galectin: implications of alternative splicing and a distinct expression profile compared to those of the three proto-type proteins

Author

José L. Saiz, Herbert Kaltner, Sabine André, Martin Lensch, Joachim C. Manning, Hans-Joachim Gabius, Michael Mürnseer, and Dolores Solís

Subjects
DNA, Complementary, Galectins, Molecular Sequence Data, Saccharomyces cerevisiae, Thymus Gland, Biology, Biochemistry, Exon, Protein structure, Complementary DNA, Gene expression, Animals, Tissue Distribution, Cloning, Molecular, Gene, Galectin, Reverse Transcriptase Polymerase Chain Reaction, Gene Expression Profiling, Macrophages, Alternative splicing, Protein Structure, Tertiary, Gene expression profiling, Alternative Splicing, Peptides, Chickens
Abstract

Animal galectins (lectins with specificity for beta-galactosides of glycan chains) are potent effectors in diverse aspects of cell sociology. Gene divergence has led to different groups and a marked interspecies variability in the number of members per group. Since the suitability of a model for studying functionality in the galectin network will be distinguished by a rather simple degree of complexity, we have focused on chicken galectins (CGs). Starting from partial expression sequence tag information, we here report on cloning of full-length cDNA for the first avian tandem-repeat-type galectin. It is termed CG-8 on the basis of its sequence similarity to galectin-8 from mammals. Systematic sequence searches revealed its unique character among CGs. Detection of two mature mRNA species points to production of isoforms. Alternative splicing affecting exon V generates the two proteins with linkers of either 9 (CG-8I) or 28 amino acids (CG-8II). Both proteins form monomers with a shape comparable to that of the proto-type proteins CG-1A/B in solution, act as cross-linkers in hemagglutination, and bind cells with a strict dependence on galactose. Western blotting revealed the presence of either CG-8II or the mixture in organ extracts. No evidence of a truncated form was obtained. Preparation of a specific antibody also enabled immunohistochemical localization. Prominent sites of its presence were defense cells in the l. propria mucosae, in addition to immune cells in distinct organs such as alveolar macrophages and thymocytes. Overall, we extend the network of CGs to a tandem-repeat-type protein and provide a detailed characterization from gene and protein structures to expression.

Published
2009

17. Detection and chromatographic removal of lipopolysaccharide in preparations of multifunctional galectins

Author

Herbert Kaltner, Martin Lensch, Kerstin Sarter, Sabine André, Connie Schulze, Hans-Joachim Gabius, Martin Herrmann, Georg Schett, and Vilma Urbonaviciute

Subjects
Lipopolysaccharides, animal structures, Lipopolysaccharide, Galectin 3, Galectins, Biophysics, Plasma protein binding, Biochemistry, Cell Line, chemistry.chemical_compound, Mice, otorhinolaryngologic diseases, medicine, Animals, Humans, Molecular Biology, Galectin, Polymyxin B, Chromatography, biology, Tumor Necrosis Factor-alpha, Lectin, Cell Biology, Dendritic Cells, biology.organism_classification, Recombinant Proteins, Bacterial adhesin, stomatognathic diseases, chemistry, Cell culture, biology.protein, lipids (amino acids, peptides, and proteins), Reagent Kits, Diagnostic, Bacteria, medicine.drug, Protein Binding
Abstract

The functional spectrum of human galectins is currently explored, with a wide range of activities being described. The role of galectin-3 as adhesin for bacteria is based on its strong binding to lipopolysaccharides (LPSs), which brings the possibility of such a contamination in galectin preparations to awareness. This assumption was verified in three independent functional assay systems using polymyxin B as inhibitor of LPS-dependent effects. Moreover, a commercial LPS quantification kit also revealed LPS in galectin preparations. Chromatography was effective in removing LPS, suggesting that such a technique needs to be applied to prevent assigning cellular responses to galectins rather than LPS.

Published
2008

18. Nuclear presence of adhesion-/growth-regulatory galectins in normal/malignant cells of squamous epithelial origin

Author

Barbora Dvořánková, Jan Motlik, Martin Lensch, Herbert Kaltner, Sabine André, Jan Bouček, Karel Smetana, Martin Chovanec, Jiří Klíma, and Hans-Joachim Gabius

Subjects
Histology, Swine, Galectins, Cell, Carbohydrates, Gene expression, medicine, Animals, Humans, Growth Substances, Molecular Biology, Galectin, Cell Nucleus, biology, Cell growth, Lectin, Cell Differentiation, Epithelial Cells, Cell Biology, Molecular biology, Squamous carcinoma, Cell biology, Gene expression profiling, stomatognathic diseases, Medical Laboratory Technology, medicine.anatomical_structure, Phenotype, Cell culture, biology.protein, Carcinoma, Squamous Cell, Cell Adhesion Molecules, Signal Transduction
Abstract

Cellular activities in the regulation of growth or adhesion/migration involve protein (lectin)-carbohydrate recognition at the cell surface. Members of the galectin family of endogenous lectins additionally bind distinct intracellular ligands. These interactions with protein targets explain the relevance of their nuclear and cytoplasmic presence. Expression profiling for galectins and accessible binding sites is a histochemical approach to link localization with cellular growth properties. Non-cross-reactive antibodies for the homodimeric (proto-type) galectins-1, -2 and -7 and the chimera-type galectin-3 (Gal-3) as well as the biotinylated lectins were tested. This analysis was performed with the FaDu squamous carcinoma cell line and long-term cultured human and porcine epidermal cells as models for malignant and normal cells of squamous cell epithelial origin. A set of antibodies was added for phenotypic cell characterization. Strong nuclear and cytoplasmic signals of galectins and the differential reactivity of labeled galectins support the notion of their individual properties. The length of the period of culture was effective in modulating marker expression. Cytochemical expression profiling is a prerequisite for the selection of distinct proteins for targeted modulation of gene expression as a step toward functional analysis.

Published
2005

19. Introduction of extended LEC14-type branching into core-fucosylated biantennary N-glycan

Author

Sabine, André, Shuji, Kojima, Ingo, Prahl, Martin, Lensch, Carlo, Unverzagt, and Hans-Joachim, Gabius

Subjects
Glycosylation, Molecular Sequence Data, Flow Cytometry, Cell Line, Epitopes, Mice, Carbohydrate Sequence, Agglutinins, Polysaccharides, Cell Line, Tumor, Lectins, Mutation, Animals, Humans, Tissue Distribution, Fucose, Glycoproteins, Protein Binding
Abstract

A series of enzymatic substitutions modifies the basic structure of complex-type biantennary N-glycans. Among them, a beta1,2-linked N-acetylglucosamine residue is introduced to the central mannose moiety of the core-fucosylated oligosaccharide by N-acetylglucosaminyltransferase VII. This so-called LEC14 epitope can undergo galactosylation at the beta1,2-linked N-acetylglucosamine residue. Guided by the hypothesis that structural modifications in the N-glycan alter its capacity to serve as ligand for lectins, we prepared a neoglycoprotein with the extended LEC14 N-glycan and tested its properties in three different assays. In order to allow comparison to previous results on other types of biantennary N-glycans the functionalization of the glycans for coupling and assay conditions were deliberately kept constant. Compared to the core-fucosylated N-glycan no significant change in affinity was seen when testing three galactoside-specific proteins. However, cell positivity in flow cytofluorimetry was enhanced in six of eight human tumor lines. Analysis of biodistribution in tumor-bearing mice revealed an increase of blood clearance by about 40%, yielding a favorable tumor/blood ratio. Thus, the extended LEC14 motif affects binding properties to cellular lectins on cell surfaces and organs when compared to the core-fucosylated biantennary N-glycan. The results argue in favor of the concept of viewing substitutions as molecular switches for lectin-binding affinity. Moreover, they have potential relevance for glycoengineering of reagents in tumor imaging.

Published
2005

20. Determination of structural and functional overlap/divergence of five proto-type galectins by analysis of the growth-regulatory interaction with ganglioside GM1 in silico and in vitro on human neuroblastoma cells

Author

Christine Fallsehr, Herbert Kaltner, Roland Russwurm, Emad Tajkhorshid, Magnus von Knebel Doeberitz, Sabine André, Hans-Joachim Gabius, Albert J. R. Heck, Martin Lensch, Juergen Kopitz, and Hans-Christian Siebert

Subjects
Models, Molecular, Cancer Research, Glycan, animal structures, Galectin 1, Galectin 2, In silico, Galectin 3, Galectins, Galectin 4, Molecular Sequence Data, G(M1) Ganglioside, Ligands, Neuroblastoma, otorhinolaryngologic diseases, Tumor Cells, Cultured, Animals, Humans, Amino Acid Sequence, Binding site, Protein Structure, Quaternary, Galectin, Ganglioside, biology, Effector, Reverse Transcriptase Polymerase Chain Reaction, Rational design, Sequence Analysis, DNA, Cell biology, Rats, stomatognathic diseases, Oncology, Biochemistry, biology.protein, Chickens, Functional divergence
Abstract

The growth-regulatory interplay between ganglioside GM1 on human SK-N-MC neuroblastoma cells and an endogenous lectin provides a telling example for glycan (polysaccharide) functionality. Galectin-1 is the essential link between the sugar signal and the intracellular response. The emerging intrafamily complexity of galectins raises the question on defining extent of their structural and functional overlap/divergence. We address this problem for proto-type galectins in this system: ganglioside GM1 as ligand, neuroblastoma cells as target. Using the way human galectin-1 interacts with this complex natural ligand as template, we first defined equivalent positioning for distinct substitutions in the other tested proto-type galectins, e.g., Lys63 vs. Leu60/Gln72 in galectins-2 and -5. As predicted from our in silico work, the tested proto-type galectins have affinity for the pentasaccharide of ganglioside GM1. In contrast to solid-phase assays, cell surface presentation of the ganglioside did not support binding of galectin-5, revealing the first level of regulation. Next, a monomeric proto-type galectin (CG-14) can impair galectin-1-dependent negative growth control by competitively blocking access to the shared ligand without acting as effector. Thus, the quaternary structure of proto-type galectins is an efficient means to give rise to functional divergence. The identification of this second level of regulation is relevant for diagnostic monitoring. It might be exploited therapeutically by producing galectin variants tailored to interfere with galectin activities associated with the malignant phenotype. Moreover, the given strategy for comparative computational analysis of extended binding sites has implications for the rational design of galectin-type-specific ligands.

Published
2004

21. Rigidified Multivalent Lactose Molecules and Their Interactions with Mammalian Galectins: A Route to Selective Inhibitors

Author

Ioannis Vrasidas, Hans-J. Gabius, Corina Böck, Martin Lensch, Rob M. J. Liskamp, Roland J. Pieters, Paola Valentini, Sabine André, and Herbert Kaltner

Subjects
chemistry.chemical_classification, Mammals, Spectrometry, Mass, Electrospray Ionization, Stereochemistry, Galectins, Organic Chemistry, Molecular Sequence Data, Lactose, General Medicine, Carbohydrate, Triple bond, Biochemistry, Folding (chemistry), chemistry.chemical_compound, Spectrometry, Fluorescence, Thiourea, Carbohydrate Sequence, chemistry, Animals, Molecule, Physical and Theoretical Chemistry, Glycoprotein, Galectin
Abstract

New and rigid multivalent lactose molecules were prepared. The structures contain lactose-2-aminothiazoline units at the periphery that were formed from a cyclisation of the thiourea sulphur onto the triple bond of the spacer. The lactosides were evaluated as inhibitors against lectin binding in a solid phase inhibition assay. In this assay the glycoprotein asialofetuin was immobilized onto the surface of microtiter plate wells, mimicking cell surface presentation, while mammalian galectins-1, -3 or -5 were in solution. Between the three galectins, the folding pattern and sequence are closely related but the topology of presentation of the carbohydrate recognition domains differs. Strong multivalency effects were observed for the tetravalent lactoside in the inhibition of galectin-3 binding with enhancements of almost 4300-fold compared to lactose. Remarkable selectivity was obtained in the inhibition since relative potencies of the tetravalent lactoside with the proto type galectins-1 and -5 did not exceed a factor of 143 relative to lactose. The binding of the lactosides to galectin-3 was also studied by fluorescence spectroscopy with all components in solution. These studies showed no multivalency effects in the inherent binding affinities.

Published
2003

22. Characterization of Chloroplast Proteases

Author

Anna Sokolenko, Martin Lensch, and Reinhold G. Herrmann

Subjects
Chloroplast, Proteases, medicine.diagnostic_test, Kinase, Chemistry, Proteolysis, Phosphatase, medicine, Efflux, Acclimatization, Cell biology, Characterization (materials science)
Abstract

As „open systems” organisms do not only add compounds (influx of matter), they also constantly exchange matter with their environment to modify structures and functions for optimization, maintenance, acclimatization, stress protection, and repair. Molecular mechanisms controlling this efflux of matter must contribute with comparable quality to the regulation of supramolecular structures as those generating them. Often such processes involve different regulatory components, such as kinases, phosphatases, or proteases, operating at various time scales that range from seconds to days.

Published
1998

23. Biomolecular engineering of human lectin galectin-2

Author

Hui Wang, Hans-Joachim Gabius, Anton P. J. Middelberg, Martin Lensch, Conan J. Fee, and Lizhong He

Subjects
biology, Chemistry, biology.protein, Lectin, Bioengineering, Biomolecular engineering, Applied Microbiology and Biotechnology, Biotechnology, Galectin, Cell biology
Published
2009

Catalog

Books, media, physical & digital resources
See catalog results