Abstract
Hemonectin is a lineage-specific cytoadhesive protein that may be involved in the developmentally regulated adhesion of granulocytic cells to bone marrow stroma. Immunoblot analysis using an anti-hemonectin antibody recognizes two distinct immunoreactive species in endothelial cell lysates (approximately M(r) 65,000) and human serum (approximately M(r) 55,000). Initial characterization of the 55-kDa protein has now been completed by isolating the cDNA from a human endothelial cell expression library. Sequence analysis of overlapping clones identifies a composite sequence spanning 2030 nucleotides with an open reading frame of 1173 base pairs. No significant sequence similarity was observed on analysis of current GenBank databases. The open reading frame was expressed as a recombinant protein in Escherichia coli and used as an immunogen for the production of a specific polyclonal antibody. Immunoblotting with this antibody identifies a single immunoreactive species of apparent M(r) 55,000 in HUVEC lysates and human serum, confirming that a secreted form normally circulates as a serum constituent protein. This antibody fails to recognize purified hemonectin, suggesting that the M(r) 55,000 protein is not hemonectin. Cross-species Southern blot analysis reveals persistent hybridizing fragments in all species tested, suggestive of a developmentally conserved function. Northern blot analysis demonstrates expression limited to endothelial and bone marrow stromal cells, but not poly(A) RNA from monkey liver, spleen, brain, lung, and kidney. On this basis, we have designated this novel protein MSE55, for marrow stromal/endothelial cell protein with a molecular mass of 55,000 daltons. Its tissue-specific expression may suggest a functional role in hematopoiesis.
Highlights
Cross-speciesSouthern blot analysis reveals persistent restricted to human endothelial and bone marrow stromal hybridizing fragmentsin all species tested, suggestive of a developmentally conserved function
Peptide sequence analysis of threetryptic fragments obtained from a purified hemonectin fraction are not contained within the primary translation product, and immunoblotting with an antibody directed against this recombinant protein fails to recognize purified hemonectin, suggesting that this protein is not hemonectin
The hematopoietic microenvironment is an elaborate meshwork of soluble growth factors, extracellular matrix (ECM),’ and stromal cells that maintains the dynamic repopulation of circulating blood elements [1].The importance of this adherent stromal cell layer in maintaining effective hematopoiesis
Summary
Plaque-purified, andthe DNA was purified from minilysates by Endothelial Cell Immunoreactivity-Human umbilical vein standard methods [14]. The initial antibody-positive cDNA insert was directly amplified from pure phage lysates by the polymerase chain reaction (X), using synthetic oligonucleotides bp upstream from the Xgtll EcoRI cloning site (forward primer 5'-TGGCTGAATATCGACGGTTTCCAT) and 79 bp downstream from the Eco RI endothelial cells were isolated and propagated as described above. A, total cellular lysates (-5 mg/ml) were gene, La Jolla, CA), and samples were size-fractionated by electro- prepared from human umbilicalvein endothelial cells (HUVEC) ( l a n e phoresis in a 0.8% agarose gel and transferred to nylon membranes 2), K562 cells (lane 3),and MOLT-4 cells ( l a n e 4 ). Ments, filters were stripped according to the manufacturer's recom- polyacrylamide gel, transferred to nitrocellulose filters, and blotted mendations, and adequacy was confirmed by overnight exposure to with the guinea pig anti-hemonectin antibody [5]a t a 1:lOOO dilution
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