Your search keyword '"Krenn V"' showing total 564 results

551. Monoclonal rat antibodies directed against Toxoplasma gondii suitable for studying tachyzoite-bradyzoite interconversion in vivo.

Author

Gross U, Bormuth H, Gaissmaier C, Dittrich C, Krenn V, Bohne W, and Ferguson DJ

Subjects

Animals, Antibodies, Monoclonal biosynthesis, Antibodies, Monoclonal classification, Antibodies, Protozoan biosynthesis, Antibodies, Protozoan classification, Antigen-Antibody Reactions, Antigens, Protozoan analysis, Fluorescent Antibody Technique, Indirect, Immunoblotting, Immunoglobulin Isotypes analysis, Immunohistochemistry, Kinetics, Mice, Mice, Inbred CBA, Rats, Species Specificity, Toxoplasmosis, Animal immunology, Toxoplasmosis, Animal parasitology, Antibodies, Monoclonal chemistry, Antibodies, Protozoan chemistry, Toxoplasma growth & development, Toxoplasma immunology

Abstract

We previously reported the in vitro analysis of stage differentiation of Toxoplasma gondii in murine bone marrow-derived macrophages. The purpose of this study was to generate monoclonal rat antibodies that might be suitable for investigating tachyzoite-bradyzoite interconversion in vivo with the murine model. Immunization of Fischer rats with cysts of T. gondii NTE resulted in the generation of seven monoclonal antibodies of the immunoglobulin G2a, G2b, or M isotype, which were further characterized by the immunoblot technique, immunofluorescence assay, immunohistology, and immunoelectron microscopy. Immunoblots demonstrated specific reactivity of five monoclonal antibodies with proteins with molecular masses of 40, 52, 55, 60, 64, 65, and 115 kDa. One antibody (CC2) appeared to recognize a differently expressed antigen depending on the parasite stage, reacting with a 40-kDa molecule in tachyzoites and a 115-kDa antigen in bradyzoites and oocysts. Several other monoclonal antibodies were shown to be stage specific and to react in immunofluorescence assays or in immunoblots with either tachyzoites or bradyzoites. Kinetics of stage conversion in vitro could be monitored by immunofluorescence with two of these monoclonal antibodies. Preliminary immunohistological investigations of tissue sections from infected mice demonstrated the possible usefulness of these monoclonal antibodies for future in vivo studies on stage differentiation of T. gondii in the murine system.

Published

1995

552. Superfetation occurring in connection with gamete intrafallopian transfer: a case report.

Author

Krenn V, Marx A, Wiedemann R, Müller-Hermelink HK, and Kranzfelder D

Subjects

Abortion, Spontaneous pathology, Adult, Female, Gestational Age, Humans, Ovarian Hyperstimulation Syndrome complications, Pregnancy, Gamete Intrafallopian Transfer, Superfetation

Abstract

This observation reports a case of susperfetation which occurred in connection with gamete intrafallopian transfer (GIFT). The macroscopic and histological examination of a spontaneous abortion from a 33-year-old woman (15th week of pregnancy) revealed the existence of two embryos with a monochorionic diamniotic placenta (developmental age approximately 41 days) and two fetuses and a fetal remnant with a trichorionic and triamniotic placenta (developmental age approximately 98 days). The large developmental age difference of embryos and fetuses cannot be explained by retardation, because the embryos showed adequate development with the development of their placenta. Moreover, the usual causes of intrauterine growth retardation could be excluded as could retention of the embryos since the tissues showed no autolytic changes. Consequently the large developmental age difference is explained by assuming that the embryos developed from successive ovulations. A second nidation of blastocysts had occurred after the GIFT concurrently with the clinically reported hyperstimulation syndrome.

Published

1995

553. Efficient immortalization of rheumatoid synovial tissue B-lymphocytes. A comparison between the techniques of electric field-induced and PEG fusion.

Author

Krenn V, von Landenberg P, Wozniak E, Kissler C, Hermelink HK, Zimmermann U, and Vollmers HP

Subjects

Animals, Antigens, CD immunology, Antigens, Differentiation, B-Lymphocyte immunology, Arthritis, Rheumatoid pathology, Electrophysiology, Humans, Hybrid Cells, Immunophenotyping, Mice, Plasma Cells cytology, Polyethylene Glycols, Sialic Acid Binding Ig-like Lectin 2, Synovial Membrane cytology, Synovial Membrane immunology, Arthritis, Rheumatoid immunology, B-Lymphocytes cytology, Cell Adhesion Molecules, Cell Fusion, Lectins

Abstract

In this study, B-cells isolated from rheumatoid synovial tissue were immortalized, without prior in vitro stimulation, by means of electric-field induced fusion and conventional PEG fusion in order to compare the efficiency of these methods. Two myeloma cell lines were used as fusion partners, the murine myeloma Ag8 and the murine-human heteromyeloma HAB-1. The results of seven fusion experiments performed simultaneously with identical cell populations showed that fusion frequencies obtained by electrofusion were 4 to 35 times higher than by the PEG fusion technique. The morphological and immunohistochemical evaluation of synovial tissues used for fusion showed that only tissues exhibiting a follicular distribution of B-cells with a high percentage of CD 22-positive lymphocytes gave rise to high fusion yields and produced B-cell clones, whereas synovial tissues with the same percentage of plasma cells but lower percentages of CD 22 lymphocytes yielded very low fusion rates. In conclusion, electrofusion is more efficient for immortalizing small amounts of synovial tissue B-lymphocytes than PEG fusion, since high fusion frequencies could be obtained by this technique without the need for prior in vitro stimulation. Synovial tissue exhibiting a follicular distribution of B-lymphocytes with high percentages of CD 22-positive lymphocytes gave rise to high hybridoma yields and therefore an ideal source of human rheumatoid B-cell clones.

Published

1995

554. Alterations of thymus cortical epithelium and interdigitating dendritic cells but no increase of thymocyte cell death in the early course of simian immunodeficiency virus infection.

Author

Müller JG, Krenn V, Schindler C, Czub S, Stahl-Hennig C, Coulibaly C, Hunsmann G, Kneitz C, Kerkau T, and Rethwilm A

Subjects

Animals, Cell Death, Dendritic Cells ultrastructure, Epithelium pathology, Flow Cytometry, Fluorescent Antibody Technique, Immunohistochemistry, In Situ Hybridization, Lymph Nodes pathology, Macaca mulatta, Microscopy, Electron, Polymerase Chain Reaction, Simian Immunodeficiency Virus, Thymus Gland ultrastructure, Time Factors, Dendritic Cells pathology, Simian Acquired Immunodeficiency Syndrome pathology, Thymus Gland pathology

Abstract

The role of the thymus in the pathogenesis of simian acquired immunodeficiency syndrome was investigated in 18 juvenile rhesus monkeys (Macaca mulatta). The thymus was infected from the first week post-SIVmac inoculation, but the amount of virus-positive cells was very low (< 1 in 10(4) T cells) as demonstrated by polymerase chain reaction and in situ hybridization. First morphological alteration was a narrowing of the cortex at 12 and 24 wpi. Morphometry revealed no increase of pyknotic T cells but a decrease of the proliferation rate and flow cytometry showed a reduction of the immature CD4+/CD8+ double-positive T cells. Ultrastructural analysis revealed vacuolization, shrinkage, and finally cytolysis of the cortical epithelial cells and the interdigitating dendritic cells. Immunofluorescence staining exhibited a widespread loss of cortical epithelial cells. This damage to the thymic microenvironment could explain the breakdown of the intrathymic T cell proliferation. It preceded fully developed simian acquired immunodeficiency syndrome and is therefore considered to play a major role in its pathogenesis.

Published

1993

555. The thymic epithelial reticulum and interdigitating cells in SIV-induced thymus atrophy and its comparison with other forms of thymus involution.

Author

Müller JG, Krenn V, Czub S, Stahl-Hennig C, Coulibaly C, Hunsmann G, and Müller-Hermelink HK

Subjects

Animals, Atrophy pathology, Disease Models, Animal, Epithelium pathology, Macaca mulatta, Microscopy, Electron, Aging pathology, Simian Acquired Immunodeficiency Syndrome complications, Simian Immunodeficiency Virus, Thymus Gland pathology

Abstract

Alterations in the thymus were investigated in the early course of SIV infection of rhesus monkeys and compared with age-related and acute accidental thymus atrophy. The SIV-induced pathology was characterized by shrinkage of the thymic parenchyma and capsule, whereas in age-related thymus atrophy, the size of the capsule remained unaltered and the emerging space was filled by fatty tissue. Acute accidental thymus involution is characterized by massive cell death of the thymocytes, but there was no increase in pycnotic thymocytes either in SIV-induced or in age-related thymus atrophy. Ultrastructural analysis revealed no major differences between the juvenile control and the aged thymus. In contrast, SIV-induced thymus atrophy exhibited severe alterations of the epithelial cells of the cortex and the interdigitating dendritic cells, which were not found in the aged thymus nor in the juvenile control cortex.

Published

1993

556. Simian immunodeficiency virus (SIV) induced alterations of thymus IDCs.

Author

Krenn V, Müller J, Mosgöller W, Czub S, Schindler C, Stahl-Hennig C, Coulibaly C, Hunsmann G, and Müller-Hermelink HK

Subjects

Animals, Atrophy, Autoimmunity, Cell Membrane ultrastructure, Cell Size, Dendritic Cells ultrastructure, Macaca mulatta immunology, Microscopy, Electron, Simian Acquired Immunodeficiency Syndrome immunology, Dendritic Cells microbiology, Simian Acquired Immunodeficiency Syndrome pathology, Simian Immunodeficiency Virus physiology, Thymus Gland pathology

Published

1993

557. Differences in the fibronectin-dependence of migrating cell populations.

Author

Brand-Saberi B, Krenn V, Grim M, and Christ B

Subjects

Animals, Antibodies, Monoclonal, Cell Differentiation, Cell Movement physiology, Chick Embryo, Coturnix embryology, Immunohistochemistry, Muscles cytology, Muscles physiology, Peptide Fragments immunology, Peptide Fragments physiology, Transplantation, Heterologous, Axons physiology, Fibronectins physiology, Melanocytes physiology, Muscles embryology, Schwann Cells physiology

Abstract

In avian embryos, the migration behaviour of several cell populations, melanoblasts, Schwann cells, myogenic cells and axons after application of antibodies directed against the cell-attachment fragment of fibronectin (alpha-CAF) was investigated. The migration of the different cell types was influenced in different ways. 1. Epidermal melanoblasts did not colonize areas into which the antibody had been injected, i.e. distal to the grafting site. They frequently spread proximally to the back and neck, sometimes even as far as to the ipsilateral leg. When grafted to the dorsal side of the wing bud, melanoblasts never spread to the ventral side after injection of the antibody. Non-epidermal melanoblasts continued to migrate distally. 2. Grafted Schwann cells and host axons were not noticeably affected by the antibody injections. Both were found proximally and far distally to the grafting site, i.e. also within the injected area. 3. Myogenic cells were immobilized near the grafting site, where they differentiated biochemically, but sometimes only partially underwent fusion into myotubes. They participated in the formation of host muscle blastemas only immediately adjacent to the non-migratory cell population of the graft such as fibroblasts and cartilage. 4. The injected antibody could be localized up to 5 h after the application in the distal third of the limb bud. We conclude that migrating cell populations show differences in their fibronectin-dependence which probably reflect their use of fibronectin during migration.

Published

1993

558. Hyaluronic acid influences the migration of myoblasts within the avian embryonic wing bud.

Author

Krenn V, Brand-Saberi B, and Wachtler F

Subjects

Animals, Cell Movement drug effects, Chick Embryo, Dextran Sulfate pharmacology, Forelimb anatomy & histology, Muscles cytology, Muscles drug effects, Coturnix embryology, Forelimb embryology, Hyaluronic Acid pharmacology, Muscles embryology

Abstract

Myoblasts migrate in a proximodistal direction within the avian embryonic wing bud during normal limb development. Since the presence and distribution of hyaluronic acid within the wing bud coincide with the time and with the direction of the migration of myoblasts, we microinjected hyaluronic acid into chicken wing buds that had received grafts containing quail myoblasts. It was found that injected hyaluronic acid has a strong positive effect on the migration of myoblasts: it causes a migration of myoblasts in donor-host combinations in which this is normally not the case, and it can cause migration in a proximal direction, a phenomenon not observed during normal development. From this it may be concluded that hyaluronic acid can influence myoblast migration in vivo. A similar effect could be observed after the microinjection of dextran sulfate, a synthetic compound having similar physicochemical properties. Hyaluronic acid, therefore, may play an important role in the control of the migration of myogenic cells in vivo by its physiocochemical properties.

Published

1991

559. [Morphological alterations of lymph nodes and thymus during the early course of SIV infection of rhesus monkeys].

Author

Müller JG, Stahl-Hennig C, Rethwilm A, Kneitz C, Kerkau T, Schmauser B, Schindler C, Krenn V, terMeulen V, and Müller-Hermelink HK

Subjects

Animals, Immunophenotyping, Macaca mulatta, Simian Acquired Immunodeficiency Syndrome physiopathology, T-Lymphocytes pathology, Time Factors, Lymph Nodes pathology, Simian Acquired Immunodeficiency Syndrome pathology, Thymus Gland pathology

Abstract

Rhesus monkeys (M. mulatta) were i.v. infected with SIV mac251. Three phases of lymph node changes were observed. 1: physiological follicular hyperplasia (3 and 6 weeks p.i.). 2: Alterations of germinal centers: loss of follicular mantle zone, fragmentation or sclerosis (12 and 24 weeks p.i.). 3: Partial depletion of T-lymphocytes, accumulation of plasma cells, increased numbers of syncytial giant cells, hemophgocytosis in the sinuses (about 1 year p.i.). The thymus of the juvenile animals showed first changes 12 and 24 weeks after infection with focal loss of immature (and Ki-67 positive) cortical thymocytes, leading to severe accidental involution of the thymuses one year after infection and reduced numbers of Hassalls corpuscles. These investigations show the value of this animal model for the study of morphology and pathogenesis of AIDS.

Published

1991

560. The orientation of the wing mesenchyme influences the direction of the migration of myoblasts in the avian embryonic wing bud.

Author

Krenn V and Wachtler F

Subjects

Animals, Cell Movement, Coturnix, Mesoderm physiology, Muscles cytology, Poultry, Muscles physiology, Wings, Animal embryology

Abstract

In order to analyze the influence of the orientation of the wing bud mesenchyme on the proximodistal direction of the migration of myoblasts in the avian embryonic wing bud, blocks of wing-bud mesenchyme were cut out and rotated around a dorso-palmar axis through 90 degrees or 180 degrees. Tissues originating from the quail wing bud and containing myoblasts were grafted into the space between the wing mesenchyme and the rotated blocks of mesenchyme proximal to the latter. In all experiments the donor-embryos were older than the acceptor-embryos. From HH stage 24 on, the rotation of the block of mesenchyme inhibited the migration of the myoblasts in a distal direction. We therefore propose that the orientation of the wing bud mesenchyme has an influence on the migratory behavior of myoblasts. This influence could provide "directional information" for the migrating myoblasts, allowing the migration of myoblasts in a distal direction only.

Published

1990

561. On the histogenetic potency of the tailbud mesoderm.

Author

Krenn V, Ostermayer H, and Wachtler F

Subjects

Animals, Cell Differentiation, Chick Embryo, Mesoderm physiology, Tail cytology, Coturnix embryology, Mesoderm cytology, Poultry embryology, Quail embryology, Tail embryology

Abstract

The caudalmost part of the tailbud mesoderm (terminal paraxial tailbud mesoderm) does not develop into somites. It is not clear whether this terminal paraxial tailbud mesoderm can be considered to be a part of the segmental plate. To elucidate the nature of the tailbud mesoderm, grafts containing caudal somites, caudal prospective somitic mesoderm and the terminal paraxial tailbud mesoderm were grafted from quail embryos into the wing bud mesoderm of chick embryos. The distinct nuclear difference between quail and chick allows the identification of the grafts on a cellular level. The grafts containing caudalmost somites and the prospective somitic mesoderm differentiate into muscle and cartilage. The terminal paraxial tailbud mesoderm, on the other hand, did not give rise to either of these tissues. From this it can be concluded that the terminal paraxial tailbud mesoderm cannot be considered to be a part of the segmental plate.

Published

1990

562. First description of mechanoreceptors in the corpus adiposum infrapatellare of man.

Author

Krenn V, Hofmann S, and Engel A

Subjects

Humans, Adipose Tissue ultrastructure, Knee anatomy & histology, Mechanoreceptors ultrastructure, Patella

Abstract

The sensory innervation of the corpus adiposum infrapatellare of the human knee joint was studied by light microscopy. Small lamellated corpuscles (pacinian corpuscles) were found in the adipose tissue of the corpus adiposum infrapatellare. The lamellated corpuscles measured about 20 microns and consisted of 3-4 lamellae. It is discussed whether the corpus adiposum infrapatellare might perform a sensory function, influencing the muscle tone via polysynaptic reflexes.

Published

1990

563. On the origin of cells determined to form skeletal muscle in avian embryos.

Author

Krenn V, Gorka P, Wachtler F, Christ B, and Jacob HJ

Subjects

Animals, Cell Differentiation, Female, Heterochromatin ultrastructure, Mitosis, Muscles embryology, Wings, Animal cytology, Coturnix embryology, Muscles cytology, Poultry embryology, Quail embryology

Abstract

Pieces of quail embryos from various developmental stages ranging from unincubated blastoderms (before the appearance of a primitive streak) to embryos having formed somites were grafted to the wing buds or into the coelomic cavity of chicken embryos. The grafts, which can be identified on a cellular level by virtue of the prominent nucleolus-associated chromatin, present in the quail and absent in the chicken, were screened after suitable periods of reincubation for the presence or absence of skeletal myotubes containing quail nuclei. Grafts having contributed to such skeletal myotubes were considered as having contained determined myogenic cells at the time of the grafting procedure. Determined myogenic cells appeared first in the primitive streak and in the mesodermal cells formed by the invagination (gastrulation) of epiblastic cells through the primitive streak. This is true for both the head process and the paraxial mesoderm. Epiblastic cells never gave rise to skeletal myotubes. Therefore it can be said, that the onset of myogenic determination coincides with gastrulation. It remains, however, to be established, whether these two events are causally related to one another.

Published

1988

564. The control of directed myogenic cell migration in the avian limb bud.

Author

Brand-Saberi B, Krenn V, and Christ B

Subjects

Animals, Chick Embryo, Hyaluronic Acid physiology, Muscles transplantation, Transplantation, Heterologous, Wings, Animal cytology, Cell Movement, Coturnix embryology, Muscles embryology, Quail embryology, Wings, Animal embryology

Abstract

Interspecific grafting experiments between chick and quail embryos were carried out in order to investigate the mechanism controlling myogenic cell migration in the avian limb bud. In six series, various experimental set-ups were prepared involving different age combinations of donor and host. The migration of the myogenic cells contained in the quail donor could be traced due to the prominent perinucleolar heterochromatin of the quail nucleus. Irrespectively of the presence or absence of the apical ectodermal ridge (AER), myogenic cells were found to migrate distally when implanted at a more distal site or into a younger host. They were even found to migrate in the reverse direction when younger host tissue was located proximal to the graft. From these findings, we conclude that the state of differentiation ("juvenility") of the limb bud mesenchyme controls the directed migration of myogenic cells.

Published

1989