Ryo Ida scite author profile

ABSTRACT. High affinity folate binding protein (HFBP) in porcine serum was purified 2,000-fold to a specific activity of 1.4 nmol of tetrahydrofolic acid (THF) bound per mg of protein, using folic acid (FA) coupled EAH-Sepharose gel affinity chromatography. Binding activity of purified HFBP to folate was examined by ultrafiltration method linked to high-performance liquid chromatography with electrochemical detection or to liquid scintillation counting. Binding affinity of HFBP to folate was characterized by dissociation constants (Kd): 13, 17, and 31 pM for tritiated FA ( 3 HFA), THF, and N 5 -methyltetrahydrofolic acid (5MF), respectively. FA, THF, and 5MF significantly inhibited binding of HFBP to 3 HFA, and according to the magnitude of intensity of the binding inhibition, the order of affinity of each folate was confirmed to be FA > THF > 5MF. Binding activity was rather high and stable for THF and 5MF at pH ranging from 6.0 to 10.0. The binding activity, however, rapidly decreased at pH below 6.0 and over 10.0. No binding activity was observed pH below 3.0 and over 12. Gel filtration analysis showed that the prepared HFBP solution had specific binding activity at around 77 kDa of apparent molecular weight, which was 82 kDa by SDS-PAGE. It is considered that this specific and stable binding enables THF to distribute in porcine plasma.-KEY WORDS: binding protein, folate, serum, swine.

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Ryo Ida

Preparation of composite catalysts composed of Pt nanoparticles and metal oxide nanosheets: Preferential formation of Pt/metal oxide interfaces

Binding Characteristics of Folate to High Affinity Folate Binding Protein Purified from Porcine Serum.

Experimental Analysis of Unsteady Phenomena on a Transonic Centrifugal Compressor with Different Upstream Pipe Geometries

Abnormal whiskers in a Persian cat resembling shaft disorder of Abyssinian cats

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