A comparison of human prothrombin, factor IX (Christmas factor), factor X (Stuart factor), and protein S

Scipio, Richard G. Di; Hermodson, Mark A.; Yates, Stanley G.; Davie, Earl W.

doi:10.1021/bi00623a022

Cited by 606 publications

(270 citation statements)

References 49 publications

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“…It is a complex glycoprotein with >50% of the carbohydrates on the activation peptide, and is also glycosylated at the C-terminus of the heavy chain (Assouline et al 1993;Inoue and Morita 1993;Di Scipio et al 1977;Cook et al 2000). The mature plasma form of factor X is a disulfide-linked two-chain molecule consisting of a light chain and a heavy chain, formed after intracellular proteolytic cleavage of the precursor (Leytus et al 1984).…”

Section: Introductionmentioning

confidence: 99%

Production of a self-activating CBM-factor X fusion protein in a stable transformed Sf9 insect cell line using high cell density perfusion culture

et al. 2004

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Factor Xa is a serine protease, whose high selectivity can be used to cleave protein tags from recombinant proteins. A fusion protein comprised of a self-activating form of factor X linked to a cellulose-binding module, saCBMFX, was produced in a stable transformed Sf9 insect cell line. The activity of the insect cell produced saCBMFX was higher than the equivalent mammalian cell produced material. A 1.5 l batch fermentation reached a maximum cell concentration of 1.6 Â 10 7 cells ml À1 and a final saCBMFX concentration of 4 mg l À1 . The production of saCBMFX by this cell line was also analyzed in a 1.5 l perfusion system using an ultrasonic filter as a cell-retention device for flow rates up to 3.5 l day À1 . The cellretention efficiency of an air backflush mode of acoustic filter operation was greater than 95% and eliminated the need to pump the relatively shear sensitive insect cells. In the perfusion system over 4 Â 10 7 Sf9 cells ml À1 were obtained with a viability greater than 80%. With a doubling of viable cell concentration from 1.5 to 3 Â 10 7 cells ml À1 the saCBMFX production rate was doubled to 6 mg l À1 day À1 . The saCBMFX volumetric productivity of the perfusion system was higher than the batch fermentations (0.6 mg l À1 day À1 ) by an order of magnitude.

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Section: Introductionmentioning

confidence: 99%

Production of a self-activating CBM-factor X fusion protein in a stable transformed Sf9 insect cell line using high cell density perfusion culture

et al. 2004

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“…Two other proteins, protein C [2] and protein S [3,4], also containing Gla residues have been isolated from blood plasma after adsorption to barium salts. An additional Glacontaining protein, protein Z, isolated from bovine plasma was initially described as a singlechain variant of factor X [5,6].…”

Section: Introductionmentioning

confidence: 99%

Isolation and N‐terminal amino acid sequence of protein Z, A γ‐carboxyglutamic acid containing protein from bovine plasma

et al. 1980

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“…It is composed of a Gla domain, two epidermal growth factor-like domains, an activation peptide, and a serine-protease domain. During blood coagulation, FX is activated by either the extrinsic pathway Factor VIIa⅐tissue factor complex or the intrinsic pathway tenase complex that comprises the phospholipidbound Factor IXa (FIXa) and activated FVIII (FVIIIa) (14). FVIIIa is a cofactor to FIXa in the activation of FX, a reaction that in many respects is very similar to the prothrombin activation (2).…”

mentioning

confidence: 99%

Defining the Factor Xa-binding Site on Factor Va by Site-directed Glycosylation

Steen¹,

Villoutreix²,

Norström³

et al. 2002

Journal of Biological Chemistry

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A comparison of human prothrombin, factor IX (Christmas factor), factor X (Stuart factor), and protein S

Cited by 606 publications

References 49 publications

Production of a self-activating CBM-factor X fusion protein in a stable transformed Sf9 insect cell line using high cell density perfusion culture

Production of a self-activating CBM-factor X fusion protein in a stable transformed Sf9 insect cell line using high cell density perfusion culture

Isolation and N‐terminal amino acid sequence of protein Z, A γ‐carboxyglutamic acid containing protein from bovine plasma

Defining the Factor Xa-binding Site on Factor Va by Site-directed Glycosylation

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