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1

Electronic Resource

The orientation of the wing mesenchyme influences the direction of the migration of myoblasts in the avian embryonic wing bud (1990)

Krenn, V. ; Wachtler, F.

Springer

Anatomy and embryology 181 (1990), S. 453-460

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ISSN: 1432-0568

Keywords: Avian ; Embryo ; Migration ; Limb mesenchyme ; Myoblasts

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 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° or 180°. 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.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02433792

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2

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Differences in the fibronectin-dependence of migrating cell populations (1993)

Brand-Saberi, B. ; Krenn, V. ; Grim, M. ; [et al.]

Springer

Anatomy and embryology 187 (1993), S. 17-26

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ISSN: 1432-0568

Keywords: Cell migration ; Neural crest ; Melanoblasts ; Myogenic cells ; Fibronectin

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 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 (α-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.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00208193

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3

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On the origin of cells determined to form skeletal muscle in avian embryos (1988)

Krenn, V. ; Gorka, P. ; Wachtler, F. ; [et al.]

Springer

Anatomy and embryology 179 (1988), S. 49-54

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ISSN: 1432-0568

Keywords: Embryo ; Quail ; Chicken ; Skeletal muscle ; Determination

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 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 cell 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.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00305099

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4

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On the histogenetic potency of the tailhud mesoderm (1990)

Krenn, V. ; Ostermayer, H. ; Wachtier, F.

Springer

Anatomy and embryology 181 (1990), S. 595-601

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ISSN: 1432-0568

Keywords: Embryo ; Quail ; Tailbud ; Differentiation

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 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.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00174631

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5

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The control of directed myogenic cell migration in the avian limb bud (1989)

Brand-Saberi, B. ; Krenn, V. ; Christ, B.

Springer

Anatomy and embryology 180 (1989), S. 555-566

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ISSN: 1432-0568

Keywords: Avian embryos ; Muscle development ; Cell migration ; Limb mesenchyme differentiation

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary 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 nor 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.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00300553

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6

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Morphological classification of nuchal skin in human fetuses with trisomy 21, 18, and 13 at 12—18 weeks and in a trisomy 16 mouse (1998)

von Kaisenberg, C. S. ; Krenn, V. ; Ludwig, M. ; [et al.]

Springer

Anatomy and embryology 197 (1998), S. 105-124

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ISSN: 1432-0568

Keywords: Key words Nuchal translucency ; Trisomy 16 ; Trisomy 21 ; Trisomy 18 ; Trisomy 13

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract An increase in the nuchal translucency that can be detected at 10–14 weeks of gestation by ultrasound forms the basis for a screening test for chromosomal abnormality. Several mechanisms leading to this increase in skin thickness have been proposed, including changes of the extracellular matrix, cardiac defects and abnormalities of the large vessels. This study examines the composition of the extracellular matrix of the skin in gestational age-matched fetuses with trisomy 21, 18 and 13 from 12–18 weeks. Immunohistochemistry was applied with monoclonal and polyclonal antibodies against collagen type I, III, IV, V and VI and against laminin and fibronectin. Collagen type VI gene expression was further studied by in situ hybridization to detect differences in expression patterns of COL6A1, COL6A3 and COL1A1 between normal fetuses and those with trisomy 21. The ultrastructure of tissue samples was studied by transmission electron microscopy (TEM) and additionally by immunogold TEM. Further, we examined the morphology of the skin in an animal model for Down’s syndrome, the murine trisomy 16, by light and TEM. The dermis of trisomy 21 fetuses was richer in collagen type VI than that of normal fetuses and other trisomies, and COL6A1, located on chromosome 21, was expressed in a wider area than COL6A3, which is located on chromosome 2. Collagen type I was less abundant in the skin of trisomy 18 fetuses, while the skin of all three trisomies contained a dense network of collagen type III and V in comparison with normal fetuses. Collagen type IV, of which two genes are located on chromosome 13, was expressed in the basement membranes of the skin in all fetuses and additionally in the dermal fibroblasts only of trisomy 13 fetuses. Likewise, laminin was present in all basement membranes of normal and trisomic fetuses as well as in dermal fibroblasts of fetuses with trisomy 18. LAMA1 and LAMA3 genes are located on chromosome 18. Dermal cysts were found in the skin of trisomy 18 and 13, but not in trisomy 21 and normal fetuses. Ultrastructural findings showed that an extracellular precipitate containing glycosaminoglycans was regularly present in the skin of trisomy 21 fetuses and murine trisomy 16 embryos. In conclusion, this study suggests that the skin edema in fetal trisomies is characterized by specific alterations of the extracellular matrix that may be attributed to gene dosage effects as a result of a genetic imbalance due to the condition of fetal trisomy.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/s004290050123

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7

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On the influence of extracellular matrix components on the myogenic cell migration in the avian wing bud

Krenn, V. ; Brans-Saberi, B.

Amsterdam : Elsevier

Cell Differentiation and Development 27 (1989), S. 66

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ISSN: 0922-3371

Source: Elsevier Journal Backfiles on ScienceDirect 1907 - 2002

Topics: Biology

Type of Medium: Electronic Resource

URL: http://linkinghub.elsevier.com/retrieve/pii/0922-3371(89)90225-6

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8

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Differential Adherence of Osteoarthritis and Rheumatoid Arthritis Synovial Fibroblasts to Cartilage and Bone Matrix Proteins and its Implication for Osteoarthritis Pathogenesis (2004)

Schedel, J. ; Wenglén, C. ; Distler, O. ; [et al.]

Oxford, UK; Malden, USA : Blackwell Science Ltd

Scandinavian journal of immunology 60 (2004), S. 0

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ISSN: 1365-3083

Source: Blackwell Publishing Journal Backfiles 1879-2005

Topics: Medicine

Notes: In osteoarthritis (OA), cartilage and bone fragments have been described within the synovial tissue which are surrounded by synovial cells (i.e. detritus synovitis). These cells appear to attach actively to the cartilage and bone fragments. In rheumatoid arthritis (RA), on the other hand, synovial fibroblasts (SF) have also been shown to be localized at sites of invasion into cartilage and bone and to degrade extracellular matrix (ECM) by secreting proteolytic enzymes. One prerequisite for exerting their aggressive properties is the attachment to cartilage and bone ECM. This attachment appears to be mediated by the expression of different adhesion molecules for which corresponding binding sites on ECM components are known. As it has not been addressed to which ECM proteins SF adhere and with which affinity this process takes place, we investigated the adherence of SF from patients with OA and RA to different cartilage and bone matrix proteins. Synovial tissue samples were obtained during synovectomy or arthroplastic surgery and used for isolating and culturing SF. Synovial cells attaching to cartilage/bone fragments were characterized using immunohistochemistry. The adherence of SF to ECM proteins was examined using an adhesion assay with the following proteins coated on 96-well plates: aggrecan (AGG), bone sialoprotein (BSP), cartilage oligomeric matrix protein (COMP), collagen type I, II and VI, proline arginine-rich, end leucine-rich repeat protein (PRELP), osteopontin (OPN) and recombinant chondroadherin (CHAD). Bovine serum albumin was used as negative control. In addition, adhering fibroblasts were photographed using a phase-contrast microscope. As compared with RA-SF, significantly higher numbers of OA-SF adhering to collagen type II, OPN and CHAD could be detected (P 〈 0.05). In contrast, RA-SF showed increased attachment to collagen type II, OPN and BSP. Adhesion to AGG, COMP and PRELP appeared not to be significantly increased and differed widely among the SF samples, and, apart from one exception (BSP), OA-SF adhered in higher numbers to the matrix proteins than did RA-SF. Using immunohistochemistry, synovial cells attached to cartilage/bone fragments could be shown to predominantly express CD68 (≥50%). The CD68-negative population was of the fibroblast phenotype (AS02 positive). The study demonstrates that the binding pattern of OA-SF and RA-SF to ECM proteins differs considerably and therefore provides novel insights into the difficult pathophysiology of OA and RA. In general, it appeared that SF adhere primarily to ECM proteins that contain known binding sites for adhesion molecules (e.g. integrins: collagen/integrin α2β1) and that higher numbers of OA-SF adhered to the cartilage and bone matrix proteins than did RA-SF.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1111/j.0300-9475.2004.01507.x

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9

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Superfetation occurring in connection with gamete intrafallopian transfer: a case report (1995)

Krenn, V. ; Marx, A. ; Müller-Hermelink, H. ; [et al.]

Springer

Virchows Archiv 426 (1995), S. 647-649

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ISSN: 1432-2307

Keywords: Superfetation ; Gamete intrafallopian transfer ; Hyperstimulation syndrome

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract This observation reports a case of superfetation 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.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00192122

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10

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Immortalized B-lymphocytes from rheumatoid synovial tissue show specificity for bacterial HSP 60 (1996)

Krenn, V. ; Vollmers, H. P. ; Landenberg, P. ; [et al.]

Springer

Virchows Archiv 427 (1996), S. 511-518

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ISSN: 1432-2307

Keywords: Rheumatoid arthritis ; Electrofusion ; Synovial B-lymphocytes ; HSP 60 ; Human monoclonal antibodies

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract Several studies indicate a pathogenetic role of T-lymphocytes with specificity for heat shock proteins (HSP) in rheumatoid arthritis (RA). Surprisingly, there are no experimental data for B-lymphocytes with specificity for HSP. To investigate whether B-lymphocytes from rheumatoid synovial tissue show a specificity for HSP 60 we immortalized synovial tissue B-lymphocytes by the electrofusion technique and tested the specificity of the B-cell clones for HSP 60 by ELISA. Tissue samples from four patients with classic, active RA were used in this study. The isolated cells were electrofused in strongly hypo-osmolar medium with cells either of the mouse strain X63-Ag8-653 (Ag8) or the heteromyeloma strain HAB-1. Clones positive for IgG, the IgG fraction of the supernatant of the isolated synovial cells and the IgG of the serum of the patients were tested in an ELISA for reactivity to the recombinant HSP 60 of Yersinia enterocolitica, which shows great homology with mycobacterial HSP 65 and human HSP 60. The expression of this HSP 60 was studied in normal and rheumatoid synovial tissue using a polyclonal rabbit serum against HSP 60 from Y. enterocolitica (Ye HSP 60). In this way we investigate differences in the expression of HSP 60 and compared the pattern of this HSP60 with the pattern of mycobacterial HSP65 and human HSP 60 described by others. In three of four patients 10 IgG secreting B-cell clones showing a specificity for HSP 60 were detected. IgG specific for HSP 60 was also detected in the supernatant of the isolated synovial cells before fusion and in the serum of these patients. HSP 60 was demonstrated immunohistochemically within the rheumatoid synovial tissue and showed stronger expression with a different distribution when compared with the expression in normal synovial tissue. B-cell clones from rheumatoid synovial tissue thus exhibit a specificity for bacterial HSP 60, and a monospecific rabbit serum against this HSP shows strong reactivity within the rheumatoid synovial tissue. It may be postulated that a humoral HSP 60 response, initially directed against an infectious agent, could react with cross-reactive epitopes of rheumatoid synovial tissue or with self-HSP perpetuating the local inflammatory process.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00199512

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