Vivienne C. Perkins scite author profile

Vivienne C. Perkins

3Publications

100Citation Statements Received

132Citation Statements Given

How they've been cited

107

How they cite others

122

Affiliations

University of Oxford

Publications

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A tumor-associated β1 integrin mutation that abrogates epithelial differentiation control

Evans

Perkins²,

Henry³

et al. 2003

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SCC4 human keratinocytes are derived from a squamous cell carcinoma of the tongue and undergo very little spontaneous differentiation. Introduction of a wild-type β1 integrin subunit into SCC4 cells stimulates differentiation, suggesting either that the cells have a defect in the integrin signaling pathways that control differentiation or that the β1 subunit itself is defective. Here we describe a heterozygous mutation in the SCC4 β1 subunit. The mutation, T188I, maps to the I-like domain. It results in constitutive activation of ligand binding, irrespective of the partner α subunit, in solid phase assays with recombinant protein and in living cells. The mutation promotes cell spreading, but not proliferation, motility, or invasiveness. It results in sustained activation of Erk MAPK independent of cell spreading. When introduced into SCC4 keratinocytes, the wild-type β1 integrin stimulates differentiation, whereas the mutant is inactive. Activation of β1 integrins in normal keratinocytes also suppresses differentiation. These results establish, for the first time, mutation as a mechanism by which integrins can contribute to neoplasia, because the degree of differentiation in epithelial cancers is inversely correlated with prognosis. They also provide new insights into how integrins regulate keratinocyte differentiation.

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Expression of a Soluble Functional Form of the Integrinα₄β₁in Mammalian Cells

Stephens¹,

Ortlepp²,

Perkins³

et al. 2000

Cell Adhesion and Communication

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The integrin a4@, (VLA4) has been expressed as a soluble, active, heterodimeric immunoglobulin fusion protein. cDNAs encoding the extracellular domains of the human a4 and PI subunits were fused to the genomic DNA encoding the human y l immunoglobulin Fc domain and functional integrin fusion protein was expressed as a secreted, soluble molecule from a range ofmammalian cell lines. Specific mutations were introduced into the Fc region of the molecules to promote '~4pI heterodimer formation. The soluble a4,9-Fc fusion protein exhibited divalent cation dependent binding to VCAM-1. which was blocked by the appropriate function blocking antibodies. The apparent Kd for VCAM-I binding were similar for both the soluble and native forms of '~4pI. In addition, the integrin-Fc fusion was shown to stain cells expressing VCAM-I on their surface by FACs analysis. This approach for expressing soluble ~4 , 6 l should be generally applicable to a range of integrins.

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Genomic Organization of the Mouse Gene for Lung Surfactant Protein D

Lawson

Perkins

Holmskov

et al. 1999

Am J Respir Cell Mol Biol

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Lung surfactant protein (SP)-D belongs to the family of soluble collagenous C-type lectins, named collectins. SP-D participates in the local innate immune defense of the lung, eliciting various effector functions by acting as a pattern recognition receptor for the carbohydrate structures on inhaled microorganisms and particulate matter. This work describes the isolation and characterization of the mouse SP-D gene (Sftpd), which spans 8 exons over 14 kb of sequence and shows an overall organization similar to other collectin genes. The complete 5' untranslated region of the messenger RNA, absent from the published complementary DNA for mouse SP-D, was also cloned and is shown to be encoded by a single exon. Analysis of 3.5 kb of 5' flanking nucleotide sequence for Sftpd is described and reveals positional conservation of a number of transcription factor binding sites on comparison of Sftpd with the human SP-D gene and the bovine conglutinin gene. In addition, a single copy SP-D-like gene has been shown to be present in mammals, birds, and amphibians but is absent in fish. An atypical, rodent-specific, long terminal repeat of retroviral origin containing a minisatellite that has become inserted in Sftpd is described. Three new polymorphic microsatellites are also described, one of which is just 160 base pairs upstream of Sftpd. This microsatellite was used to map the gene to the central region of chromosome 14; fine-scale mapping indicates that it lies in a 5. 64-centimorgan area between D14Mit45 and D14Mit60. This will allow the easy identification of the collectin gene cluster and aid in the construction of a physical map over this region.

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