Search

Your search keyword '"Kariniemi AL"' showing total 20 results
Start Over Author "Kariniemi AL" Search Limiters Available in Library Collection
20 results on '"Kariniemi AL"'

4. A retrospective study of the probability of the evolution of parapsoriasis en plaques into mycosis fungoides.

Author

Väkevä L, Sarna S, Vaalasti A, Pukkala E, Kariniemi AL, and Ranki A

Subjects
Adult, Aged, Cell Transformation, Neoplastic, Cohort Studies, Female, Finland epidemiology, Humans, Male, Middle Aged, Mycosis Fungoides drug therapy, Mycosis Fungoides pathology, PUVA Therapy, Psoriasis pathology, Registries, Retrospective Studies, Skin Neoplasms drug therapy, Skin Neoplasms pathology, Mycosis Fungoides epidemiology, Mycosis Fungoides etiology, Psoriasis complications, Skin Neoplasms epidemiology, Skin Neoplasms etiology
Abstract

Parapsoriasis en plaque has been suggested to be an early manifestation of mycosis fungoides (cutaneous T-cell lymphoma). We explored the disease course of patients with small plaque or large plaque parapsoriasis in a 26-year retrospective cohort analysis of 105 parapsoriasis patients, who were clinically and histopathologically followed up in Helsinki and Tampere University Hospitals. Eventual later cancers of these patients were verified from the Finnish Cancer Registry. In the small plaque parapsoriasis group, 7 patients (10%) and in the large plaque parapsoriasis group 12 patients (35%), developed histologically confirmed mycosis fungoides during a median of 10 and 6 years, respectively. No significant differences were found regarding the risk of developing mycosis fungoides or the tendency to remission in patients treated with or without phototherapy. Our results show that not only large plaque parapsoriasis, but also small plaque parapsoriasis, as currently defined in textbooks, can progress to mycosis fungoides. The benefits of phototherapy are equivocal in parapsoriasis treatment as far as progression to cancer is concerned.

Published
2005
Full Text
View/download PDF

5. HCR, a candidate gene for psoriasis, is expressed differently in psoriasis and other hyperproliferative skin disorders and is downregulated by interferon-gamma in keratinocytes.

Author

Suomela S, Elomaa O, Asumalahti K, Kariniemi AL, Karvonen SL, Peltonen J, Kere J, and Saarialho-Kere U

Subjects
Adult, Bowen's Disease genetics, Bowen's Disease metabolism, Carcinoma, Basal Cell genetics, Carcinoma, Basal Cell metabolism, Cell Division, Cells, Cultured, Down-Regulation, Gene Expression drug effects, Humans, Intracellular Signaling Peptides and Proteins, Keratinocytes cytology, Paget's Disease, Mammary genetics, Paget's Disease, Mammary metabolism, Psoriasis metabolism, Skin Neoplasms genetics, Skin Neoplasms metabolism, Antineoplastic Agents pharmacology, Interferon-gamma pharmacology, Keratinocytes physiology, Proteins genetics, Proteins metabolism, Psoriasis genetics
Abstract

We have previously shown that HCR is a good candidate gene for psoriasis based on its location in the PSORS1 locus, predicted secondary structure change of the associated allele, and expression pattern. To understand better the function of HCR, we studied how HCR expression is altered in hyperproliferative skin diseases other than psoriasis and in cancers. We examined also its regulation by different cytokines, growth factors, and antipsoriatic agents using quantitative RT-PCR (TaqMan) analysis and its location by immunostaining of keratinocyte cultures. Compared to psoriasis, HCR protein had a different distribution in chronic dermatitis, pityriasis rubra pilaris, mycosis fungoides, and chronic skin ulcers. In three of six grade III squamous cell carcinomas of the skin, four of four adenocarcinomas of the lung, and two of two ductal breast adenocarcinomas, positive cytoplasmic staining in cancer cells was detected. As in psoriasis, Ki67 did not colocalize with HCR. In cell cultures, HCR staining was detected perinuclearly in the cytoplasm and in the nuclei, suggesting that the protein may have a role in both compartments. A 2-fold downregulation of HCR mRNA expression was observed on stimulation with interferon-gamma. Based on the observations that HCR is detected in cancers of epithelial origin in Ki67-negative areas and that interferon-gamma downregulates its expression, we suggest it to have an antiproliferative function.

Published
2003
Full Text
View/download PDF

6. Matrix metalloproteinase-19 is expressed by keratinocytes in psoriasis.

Author

Suomela S, Kariniemi AL, Impola U, Karvonen SL, Snellman E, Uurasmaa T, Peltonen J, and Saarialho-Kere U

Subjects
Basement Membrane physiology, Cell Division physiology, Humans, Lichen Planus metabolism, Lichen Planus pathology, Lichenoid Eruptions metabolism, Lichenoid Eruptions pathology, Matrix Metalloproteinases biosynthesis, Matrix Metalloproteinases, Secreted, Psoriasis pathology, Keratinocytes metabolism, Metalloendopeptidases biosynthesis, Psoriasis metabolism
Abstract

Keratinocyte hyperproliferation, inflammatory infiltrates, neoangiogenesis and alterations in cytokine levels are hallmarks of psoriatic skin. Matrix metalloproteinases (MMPs) have been associated with the remodeling of the extracellular matrix during inflammation, neovascularization, and malignant transformation. We have previously shown that particularly MMP-12 is abundantly expressed by macrophages and MMP-9 in macrophages and neutrophils of psoriatic lesions. In this work the expression of two novel metalloproteinases, MMP-19 and MMP-28, was investigated in psoriatic lesional and non-lesional skin. MMP-19 protein was detected by immunohistochemistry in 28/29 samples in keratinocytes in the same regions as Ki67 (marker of proliferating keratinocytes) and p63 (marker of keratinocyte stem cells). Immunosignaling was also seen in endothelial cells and fibroblasts. Furthermore, MMP-19 mRNA was upregulated in psoriatic keratinocytes and skin as assessed by quantitative real-time polymerase chain reaction. In lichen planus and lichenoid chronic dermatitis, MMP-19 staining was found in keratinocytes in areas where the basement membrane was abnormal. MMP-28 was not detected in psoriatic or non-lesional skin. Our results suggest that keratinocytes as well as the previously reported cell types (smooth muscle, endothelial and macrophages) can express MMP-19 in psoriasis and lichen planus. Upregulation of MMP-19 in keratinocytes may be influenced by changes in the architecture of the basement membrane zone.

Published
2003
Full Text
View/download PDF

8. Expression of collagenases-1 and -3 and their inhibitors TIMP-1 and -3 correlates with the level of invasion in malignant melanomas.

Author

Airola K, Karonen T, Vaalamo M, Lehti K, Lohi J, Kariniemi AL, Keski-Oja J, and Saarialho-Kere UK

Subjects
Adult, Aged, Aged, 80 and over, Blotting, Northern, Disease Progression, Female, Gelatin, Gelatinases biosynthesis, Gelatinases metabolism, Humans, Male, Matrix Metalloproteinase 1, Matrix Metalloproteinase 13, Matrix Metalloproteinase 2, Matrix Metalloproteinase Inhibitors, Melanoma metabolism, Metalloendopeptidases biosynthesis, Metalloendopeptidases metabolism, Middle Aged, Neoplasm Invasiveness, Tumor Cells, Cultured, Collagenases biosynthesis, Melanoma enzymology, Melanoma pathology, Tissue Inhibitor of Metalloproteinase-1 biosynthesis, Tissue Inhibitor of Metalloproteinase-3 biosynthesis
Abstract

Since proteolysis of the dermal collagenous matrix and basement membranes is required for local invasive growth and early metastasis formation of cutaneous melanomas, we have analysed the activities/expression levels of certain metalloproteinases in melanomas and cultured melanoma cells by in situ hybridization and Northern analysis. In addition to collagenases-1 and -3 that have been implicated in invasive growth behaviour of various malignant tumours, we analysed the levels of 72-kDa gelatinase and its activators MT1-MMP and TIMP-2 in cultured melanoma cells. The lesions examined included three cases of lentigo maligna and 28 cases of Clark grade I-V melanomas. The premalignant as well as the grade I tumours were consistently negative for collagenase-1 and -3 and TIMP-1 and -3. The collagenases were predominantly expressed in the cancer cells of Clark grade III and IV tumours. TIMP-1 and -3 were abundantly expressed in the cancer and/or stromal cells of grade III and IV melanomas, while TIMP-2 protein was detected also in melanomas representing lower invasive potential. Northern analysis of seven melanoma cell lines showed that the expression of collagenase-1 and TIMPs-1 and -3 was associated with 72-kDa gelatinase positivity. All melanoma cell lines were positive for MT1-MMP and TIMP-2 mRNAs. Our results suggest that overexpression of collagenases-1 and -3 and TIMPs-1 and -3 is induced during melanoma progression. Expression of TIMPs may reflect host response to tumour invasion in an effort to control MMP activity and preserve extracellular matrix integrity.

Published
1999
Full Text
View/download PDF

9. Enhanced expression of human metalloelastase (MMP-12) in cutaneous granulomas and macrophage migration.

Author

Vaalamo M, Kariniemi AL, Shapiro SD, and Saarialho-Kere U

Subjects
Cell Movement, Collagenases analysis, Dermatitis Herpetiformis metabolism, Granuloma pathology, Granuloma Annulare metabolism, Humans, Matrix Metalloproteinase 12, Matrix Metalloproteinase 9, Metalloendopeptidases analysis, Necrobiosis Lipoidica metabolism, Pityriasis Lichenoides metabolism, RNA, Messenger analysis, Sarcoidosis metabolism, Skin Diseases pathology, Granuloma metabolism, Macrophages physiology, Metalloendopeptidases genetics, Skin Diseases metabolism
Abstract

Accumulation of inflammatory cells such as macrophages may lead to degeneration of connective tissue matrix in various skin diseases. Macrophage metalloelastase, is a matrix metalloproteinase (MMP-12) capable of degrading elastin as well as various basement membrane components. To investigate the role of human macrophage metalloelastase in skin, we assessed by in situ hybridization and immunohistochemistry 66 specimens representing skin diseases characterized either by changes in elastic fibers or by pronounced infiltrations of extravasating and migrating macrophages. CD68 immunostaining was performed to identify the human macrophage metalloelastase-positive cells and Weigert's Resorcin-Fuchsin staining to reveal the status of elastic fibers. We found abundant expression of human macrophage metalloelastase mRNA in macrophages in areas devoid of normal elastic fibers in granulomatous skin diseases sarcoidosis, necrobiosis lipoidica diabeticorum, and granuloma annulare. Positive cells for human macrophage metalloelastase protein could be detected in the same regions as well as positive immunostaining for urokinase plasminogen activator. Of the other matrix metalloproteinases capable of degrading elastin, 92 kDa gelatinase colocalized with human macrophage metalloelastase, while 72 kDa gelatinase was produced by surrounding fibroblast-like cells. Furthermore, human macrophage metalloelastase was expressed by macrophages in areas with disrupted basement membrane, as assessed by type IV collagen staining, in pityriasis lichenoides and dermatitis herpetiformis. Specimens of anetoderma, acrodermatitis chronica atrophicans and pseudoxanthoma elasticum showed no signal for human macrophage metalloelastase. Matrilysin was not detected in any of the samples investigated. Our study suggests that human macrophage metalloelastase may contribute to elastin degradation occurring in granulomatous skin diseases and may aid macrophage migration through the epidermal and vascular basement membranes in inflammatory disorders.

Published
1999
Full Text
View/download PDF

10. Human collagenase-3 is expressed in malignant squamous epithelium of the skin.

Author

Airola K, Johansson N, Kariniemi AL, Kähäri VM, and Saarialho-Kere UK

Subjects
Basement Membrane chemistry, Carcinoma, Basal Cell enzymology, Carcinoma, Basal Cell genetics, Carcinoma, Squamous Cell enzymology, Cell Adhesion Molecules analysis, Collagen analysis, Collagenases physiology, Epithelium enzymology, Extracellular Matrix metabolism, Gene Expression, Genetic Markers physiology, Head and Neck Neoplasms enzymology, Humans, Immunohistochemistry, Matrix Metalloproteinase 13, Matrix Metalloproteinase 3 genetics, Paget Disease, Extramammary enzymology, Paget Disease, Extramammary genetics, Precancerous Conditions genetics, RNA Probes analysis, RNA, Messenger metabolism, Skin enzymology, Skin Neoplasms enzymology, Kalinin, Carcinoma, Squamous Cell genetics, Collagenases genetics, Head and Neck Neoplasms genetics, Skin Neoplasms genetics
Abstract

Co-expression of several members of the matrix metalloproteinase (MMP) family is a characteristic of human carcinomas. To investigate the role of the recently cloned collagenase-3 (MMP-13) in epidermal tumors, we studied samples representing malignant (basal and squamous cell carcinoma, Paget's disease), pre-malignant (Bowen's disease, solar keratosis), and benign (keratoacanthoma, seborrheic keratosis, linear epidermal nevus) tumors. Basal cell carcinomas expressed collagenase-3 mRNA in focal areas of keratinized cells, the squamous differentiation of which was confirmed by positive immunostaining for involucrin. Apoptosis was observed in central parts of these foci. In squamous cell carcinomas, collagenase-3 expression was detected at the epithelial tumor front and less frequently in the surrounding stromal cells. Collagenase-3 mRNA co-localized with immunostaining for laminin-5, an adhesion molecule suggested to participate in the migration of tumor cells. The pre-malignant and benign tumors were mostly negative for collagenase-3. Stromelysin-1, a potential activator of latent collagenases, was frequently expressed by stromal cells surrounding the malignant tumors, and the two MMPs occasionally co-localized in keratotic foci. Our results demonstrate that in basal cell carcinomas, expression of collagenase-3 is associated with terminal differentiation of epithelial cells. Furthermore, the gene is activated during skin carcinogenesis, and we suggest a role for collagenase-3 in degradation of the extracellular matrix associated with malignant epithelial growth.

Published
1997
Full Text
View/download PDF

11. Expression of collagenase-3 (matrix metalloproteinase-13) in squamous cell carcinomas of the head and neck.

Author

Johansson N, Airola K, Grénman R, Kariniemi AL, Saarialho-Kere U, and Kähäri VM

Subjects
Adult, Aged, Aged, 80 and over, Collagenases analysis, Female, Humans, In Situ Hybridization, Male, Matrix Metalloproteinase 13, Middle Aged, RNA, Messenger analysis, Tumor Cells, Cultured, Carcinoma, Squamous Cell enzymology, Collagenases biosynthesis, Head and Neck Neoplasms enzymology
Abstract

Squamous cell carcinomas (SCCs) of the head and neck are malignant tumors with high capacity to invade and metastasize. We have examined expression of the new collagenase, collagenase-3 (MMP-13), in SCCs of the head and neck. MMP-13 mRNAs were detected in 22 of 29 SCC cell lines: in 14 of 15 primary SCC cell lines and in 8 of 14 SCC cell lines from recurrent tumors or metastases. MMP-13 mRNAs were expressed by all 6 cell lines from highly invasive primary tumors and in all 4 cell lines from small aggressive tumors. Using in situ hybridization, MMP-13 mRNAs were detected in 15 of 17 SCC tumor samples. In most tumors, MMP-13 was expressed by tumor cells at the invading front of the tumors, but in a subset of SCCs, MMP-13 mRNA was also expressed by stromal fibroblasts. No MMP-13 expression was detected in intact skin or oral mucosa. MMP-13 mRNA levels in SCC cells were enhanced by transforming growth factor-beta, tumor necrosis factor-alpha, transforming growth factor-alpha, and keratinocyte growth factor. Specific expression of MMP-13 by SCC cells in vitro and in vivo strongly suggests a role for MMP-13 in the high invasion capacity of SCC cells.

Published
1997

12. Distinct populations of stromal cells express collagenase-3 (MMP-13) and collagenase-1 (MMP-1) in chronic ulcers but not in normally healing wounds.

Author

Vaalamo M, Mattila L, Johansson N, Kariniemi AL, Karjalainen-Lindsberg ML, Kähäri VM, and Saarialho-Kere U

Subjects
Cell Count, Chronic Disease, Fibroblasts cytology, Gene Expression, Humans, In Situ Hybridization, Leg Ulcer, Matrix Metalloproteinase 1, Matrix Metalloproteinase 13, Skin Ulcer, Stromal Cells, Collagenases genetics, Skin cytology, Wound Healing genetics
Abstract

Proteolysis is an intrinsic component of cutaneous wound repair and several matrix metalloproteinases have been shown to participate in various stages of this process. Therefore, we investigated the expression of a novel metalloproteinase, collagenase-3 (MMP-13), in normally healing cutaneous wounds and chronic venous ulcers. MMP-13 was expressed abundantly by fibroblasts deep in the chronic ulcer bed but was not detected in epidermis and all the acute wounds. The spatial expression of MMP-13 differed from that of collagenase-1 (MMP-1), which was prominently expressed by migrating keratinocytes and dermal cells located just beneath the wound surface. Northern blot hybridization did not reveal expression of MMP-13 by fibroblasts cultured on tissue culture plastic. In accordance with our in vivo findings, however, fibroblasts grown in a collagen gel produced MMP-13 mRNA abundantly. Our results suggest that MMP-13 can be induced in skin during wound repair after altered cell-matrix interactions. Although both MMP-1 and MMP-13 have the unique ability to degrade fibrillar collagens, their regulation and role during wound repair seem different. Collagenase-1 is critical for re-epithelialization, and MMP-13 most likely plays a role in the remodeling of collagenous matrix in chronic wounds.

Published
1997
Full Text
View/download PDF

14. Integrins in human cells and tumors.

Author

Virtanen I, Korhonen M, Kariniemi AL, Gould VE, Laitinen L, and Ylänne J

Subjects
Animals, Cells, Cultured, Embryonic and Fetal Development, Humans, Integrins analysis, Kidney chemistry, Kidney embryology, Melanoma, Experimental pathology, Mice, Neoplasm Proteins analysis, Neoplasms physiopathology, Tumor Cells, Cultured, Cell Adhesion, Extracellular Matrix Proteins metabolism, Integrins physiology, Neoplasm Proteins physiology, Neoplasms chemistry
Abstract

We have studied the distribution of the alpha- and beta-subunits of integrins in developing and adult human kidney as well as in selected other tissues and cultured cells. In cultured cells some of the integrin subunits (beta 1, alpha 1, alpha 2 and alpha 5) colocalize with talin at focal adhesions when plated on an appropriate ligand. Similarly, in tissues the polarization of beta 1-integrins in colocalization with talin appears to indicate adhesive complexes, as demonstrated in adult glomeruli. In human kidney, the alpha subunits of integrins were seen to be segment-specifically expressed already in fetal tissues. In glomeruli the integrin alpha 1 subunit characterized mesangial cells while the alpha 2 and alpha 3 subunits showed immunoreactivity in endothelial cells and podocytes, respectively. In renal tubuli, the alpha 6 subunit, complexed with the beta 1 subunit, showed a typical polarized distribution coaligning with the tubular basement membrane while the alpha 3 and alpha 2 subunits were expressed in distal tubular cells. These results suggested that in kidney the alpha 2 beta 1, alpha 3 beta 1, and alpha 6 beta 1 integrins can function as basement membrane receptors. The alpha 5 subunit was nearly lacking in the kidney and it appears to be mainly expressed in some smooth muscle cells. In other tissues distinct patterns in the expression of integrins were found. Thus, in many glandular epithelial cells the alpha 3 beta 1 integrin appeared to function as a basement membrane receptor while in various stratified epithelia and in the breast such a polarized localization could be found for the alpha 6 beta 4 integrin. Finally, although presenting a clearly polarized distribution for beta 1 integrins, none of the alpha subunits could be found in cardiac or skeletal muscle cells and none of the integrins could be revealed in neuronal cells of human developing and adult cerebrum or cerebellum, although neurons in peripheral tissues contained abundantly the alpha 6 beta 1 integrin complex. In human tumors, the tumor cells, including also metastastatic tumors, generally presented the same integrins as their tissues of origin. In some poorly differentiated tumors both a population heterogeneity and even a lack of expression or a disorganization of basement membrane receptor integrins was obvious.

Published
1990
Full Text
View/download PDF

15. Epidermis is the origin of high creatine kinase levels in skin blister fluid.

Author

Kiistala U, Paavonen T, Saarelainen I, Aronen H, Asko-Seljavaara S, Kariniemi AL, Ingervo L, and Niemitalo S

Subjects
Biopsy, Cell Count, Cells, Cultured, Epidermis pathology, Humans, Isoenzymes, Middle Aged, Blister enzymology, Creatine Kinase biosynthesis, Epidermis enzymology
Abstract

Creatine kinase (CK) isoenzyme, CK-BB, known as the brain fraction, is not normally present in serum but predominates in several normal and malignant tissues and body fluids. We recently reported increased CK-BB levels in suction blister fluid. In the present study the cellular origin of the enzyme in skin was studied from homogenates of blister top epidermis and blister base dermis as well as from homogenates of split skin dermatome shavings and isolated keratinocytes. The CK-BB in human skin was derived almost exclusively from the epidermis. Enzyme determinations from various spontaneous bullae suggest that all types of skin blisters initially contain high CK-BB levels.

Published
1989

16. Fluorochrome-coupled lectins reveal distinct cellular domains in human epidermis.

Author

Virtanen I, Kariniemi AL, Holthöfer H, and Lehto VP

Subjects
Adult, Binding Sites, Blood Group Antigens, Epidermal Cells, Epidermis metabolism, Fetus, Fluorescent Antibody Technique, Humans, Microscopy, Fluorescence, Skin cytology, Fluorescent Dyes, Lectins, Skin metabolism
Abstract

The distribution of saccharide moieties in human interfollicular epidermis was studied with fluorochrome-coupled lectins. In frozen sections Concanavalin A (Con A), Lens culinaris agglutinin (LCA), Ricinus communis agglutinin I (RCAI), and wheat germ agglutinin (WGA) stained intensively both dermis and viable epidermal cell layers, whereas peanut agglutinin (PNA) bound only to living epidermal cell layers. Ulex europaeus agglutinin I (UEAI) bound to dermal endothelial cells and upper cell layers of the epidermis but left the basal cell layer unstained. Dolichos biflorus agglutinin (DBA) bound only to basal epidermal cells, whereas both soybean agglutinin (SBA) and Helix pomatia agglutinin (HPA) showed strong binding to the spinous and granular cell layers. On routinely processed paraffin sections, a distinctly different staining pattern was seen with many lectins, and to reveal the binding of some lectins a pretreatment with protease was required. All keratin-positive cells in human epidermal cell suspensions, obtained with the suction blister method, bound PNA, whereas only a fraction of the keratinocytes bound either DBA or UEAI. Such a difference in lectin binding pattern was also seen in epidermal cell cultures both immediately after attachment and in organized cell colonies. This suggests that in addition to basal cells, more differentiated epidermal cells from the spinous cell layer are also able to adhere and spread in culture conditions. Gel electrophoretic analysis of the lectin-binding glycoproteins in detergent extracts of metabolically labeled primary keratinocyte cultures revealed that the lectins recognized both distinct and shared glycoproteins. A much different lectin binding pattern was seen in embryonic human skin: fetal epidermis did not show any binding of DBA, whereas UEAI showed diffuse binding to all cell layers but gave a bright staining of dermal endothelial cells. This was in contrast to staining results obtained with a monoclonal cytokeratin antibody, which showed the presence of a distinct basal cell layer in fetal epidermis also. The results indicate that expression of saccharide moieties in human epidermal keratinocytes is related to the stage of cellular differentiation, different cell layers expressing different terminal saccharide moieties. The results also suggest that the emergence of a mature cell surface glycoconjugate pattern in human epidermis is preceded by the acquisition of cell layer-specific, differential keratin expression.

Published
1986
Full Text
View/download PDF

17. Disseminated superficial "actinic" porokeratosis.

Author

Kariniemi AL, Kotovirta ML, and Stubb S

Subjects
Aged, Female, Humans, Keratosis pathology, Skin pathology, Keratosis genetics
Abstract

An 81-year-old Finnish female had a 10-month history of a very pruritic eruption. In the clinical examination porokeratosis was suspected and histologically verified with the typical cornoid lamellae. The eruption involved also the unexposed areas of the skin. The patient had always avoided sunshine because it made her feel uncomfortable. The patient's sister, too, had a solitary lesion of porokeratosis. The pathomechanism of DSAP is discussed.

Published
1979

18. Dolichos biflorus agglutinin (DBA) reacts selectively with mast cells in human connective tissues.

Author

Hormia M, Kariniemi AL, Laitinen L, and Virtanen I

Subjects
Breast, Fluorescein-5-isothiocyanate, Fluoresceins, Gastric Mucosa, Gingiva, Humans, Intestinal Mucosa, Mast Cells analysis, Microscopy, Fluorescence, Thiocyanates, Connective Tissue metabolism, Lectins metabolism, Mast Cells metabolism, Plant Lectins
Abstract

Dolichos biflorus agglutinin (DBA) binds to N-acetyl-D-galactosamine (GalNAc) residues in glycoconjugates and agglutinates erythrocytes carrying blood group antigen A. In cryostat sections of various tissues from blood group-specified humans, fluorochrome-coupled DBA bound preferentially to fusiform connective tissue cells and to certain epithelial cells. The connective tissue cells were identified as mast cells by their typical metachromasia in consecutive staining with toluidine blue. Double labeling with DBA and conjugated avidin revealed two distinct populations of mast cells. In several tissues the DBA-reactive cells likewise displayed uniform avidin reactivity. In intestinal mucosa, however, morphologically distinct DBA-binding mast cells were found, which were labeled with the avidin conjugates only in specially fixed paraffin sections. DBA did not bind to vascular endothelial cells, which could be identified by double staining with antibodies to factor VIII-related antigen. Labeling with Helix pomatia agglutinin (HPA), another blood group A-reactive lectin, resulted in distinct blood group-dependent fluorescence of the endothelia. Sophora japonica agglutinin (SJA), a blood group B-reactive lectin, labeled vascular endothelial cells in tissues from blood group A, AB, and B donors. HPA and SJA reacted with small mast cells in the gastrointestinal mucosa but failed to label large mast cells in any of the tissues. These results indicate that the blood group reactivity of lectins, as determined by erythroagglutination, is not necessarily consistent with their reactivity with blood group determinants in tissue sections. Moreover, DBA conjugates appear to be a reliable probe for detection of mast cells in various human connective tissues.

Published
1988
Full Text
View/download PDF

19. Cytoskeleton and pericellular matrix organization of pure adult human keratinocytes cultured from suction-blister roof epidermis.

Author

Kariniemi AL, Lehto VP, Vartio T, and Virtanen I

Subjects
Adolescent, Adult, Blister, Cell Adhesion, Cell Division, Cells, Cultured, Epidermal Cells, Fibronectins analysis, Humans, Intermediate Filament Proteins analysis, Keratins analysis, Microscopy, Fluorescence, Middle Aged, Peptide Biosynthesis, Vimentin, Skin cytology
Abstract

Pure adult human keratinocyte cultures were raised from suction-blister roof epidermis and cultured in MCDB-151 medium. In primary culture the epidermal cells rapidly adhered, spread and began to proliferate on collagen-coated growth substrata but not on uncoated plastic or glass substrata. A fibrillar keratin-specific fluorescence, showing a typical cell-cell arrangement, was seen in all cells in indirect immunofluorescence microscopy, whereas only some cells also showed vimentin-specific staining. A fine fibrillar fibronectin-specific surface staining was seen at the margin of attaching cells and in marginal cells of spreading cell islands, whereas no fluorescence could be seen in epidermal cells, with antibodies against type IV collagen or laminin. Interestingly, the marginal cells also showed intracellular fibronectin. The synthesis of fibronectin in epidermal cell cultures could also be revealed by metabolic labelling experiments with [35S]methionine. In contrast to primary cultures, subcultivated keratinocytes also adhered to uncoated plastic and glass substrata. After subcultivation, keratin and surface fibronectin distribution remained unaltered but after some subcultivations, most of the cells also showed fibrillar vimentin and expressed fibronectin intracellularly. The results show that the suction-blister method provides an easy way to obtain pure epidermal cell cultures without contaminating mesenchymal cells. Our results also suggest a direct role for fibronectin but not for collagen type IV or laminin in adhesion and spreading of epidermal cells in vitro.

Published
1982
Full Text
View/download PDF

Catalog

Books, media, physical & digital resources
See catalog results