Your search keyword '"1000070197622"' showing total 2 results

1. Novel monoclonal antibody recognizing triglyceride-rich oxidized LDLs associated with severe liver disease and small oxidized LDLs in normal subjects

Author

Sakurai, Toshihiro, Ichikawa, Ayako, Furukawa, Hiroyuki, Wada, Norio, Nagasaka, Atsushi, Takahashi, Yuji, Fujikawa, Masato, Ikuta, Akiko, Furumaki, Hiroaki, Shiga, Maiko, 1000000292029, Shimizu, Chikara, 1000090337030, Hui, Shu-Ping, Jin, Shigeki, 1000080374726, Takeda, Seiji, Fuda, Hirotoshi, Nagasaka, Hironori, 1000030150246, Kobayashi, Seiichi, 1000070197622, Chiba, Hitoshi, Sakurai, Toshihiro, Ichikawa, Ayako, Furukawa, Hiroyuki, Wada, Norio, Nagasaka, Atsushi, Takahashi, Yuji, Fujikawa, Masato, Ikuta, Akiko, Furumaki, Hiroaki, Shiga, Maiko, 1000000292029, Shimizu, Chikara, 1000090337030, Hui, Shu-Ping, Jin, Shigeki, 1000080374726, Takeda, Seiji, Fuda, Hirotoshi, Nagasaka, Hironori, 1000030150246, Kobayashi, Seiichi, 1000070197622, and Chiba, Hitoshi

Abstract

Background: Triglyceride-rich low-density lipoproteins (TG-rich LDLs) in the plasma of patients with severe liver disease are reported to change macrophages into foam cells in vitro. Methods: Male BALB/c mice were immunized with TG-rich LDLs isolated from the plasma of a patient with severe liver disease. The resulting monoclonal antibody (G11-6) was used in a sandwich enzyme-linked immunosorbent assay (ELISA) in combination with polyclonal anti-apolipoprotein B antibodies. The time course of copper-mediated LDL oxidation was monitored using this ELISA. The results were compared to those of the two commercial ELISAs for oxidized LDL using DLH or ML25, thiobarbituric acid reactive substances (TBARS), and the optical absorbance for the conjugated dienes generated in lipid peroxides. Further, the lipoprotein fractions separated by gel filtration were tested with this ELISA in healthy volunteers (n = 11) and patients (n = 3) with liver disease. Results: G11-6 reacted with oxidized LDLs during only the early phase of copper-oxidation, being distinct from the other monoclonal antibodies and methods. G11-6 was confirmed to react with TG-rich LDLs in patients, while it reacted with small LDL particles in normal controls. Conclusions: The monoclonal antibody G11-6 is useful for detecting oxidized small LDLs in normal controls and oxidized TG-rich LDLs in patients with severe liver disease.

Published

2012

2. Measurement of lipoprotein particle sizes using dynamic light scattering

Author

Sakurai, Toshihiro, Trirongjitmoah, Suchin, Nishibata, Yuka, Namita, Takeshi, Tsuji, Masahiro, 1000090337030, Hui, Shu-Ping, Jin, Shigeki, 1000030125322, Shimizu, Koichi, 1000070197622, Chiba, Hitoshi, Sakurai, Toshihiro, Trirongjitmoah, Suchin, Nishibata, Yuka, Namita, Takeshi, Tsuji, Masahiro, 1000090337030, Hui, Shu-Ping, Jin, Shigeki, 1000030125322, Shimizu, Koichi, 1000070197622, and Chiba, Hitoshi

Abstract

Background: A simple method for the measurement of LDL particle sizes is needed in clinical laboratories because a predominance of small dense LDL (sd LDL) has been associated with coronary heart disease. We applied dynamic light scattering (DLS) to measure lipoprotein particle sizes, with special reference to sd LDL. Methods: Human serum lipoproteins isolated by a combination of ultracentrifugation and gel chromatography, or by sequential ultracentrifugation, were measured for particle size using DLS. Results: The sizes of polystyrene beads, with diameters of 21 and 28 nm according to the manufacturer, were determined by DLS as 19.3 ± 1.0 nm (mean ± SD, n = 11) and 25.5 ± 1.0 nm, respectively. The coefficients of variation for the 21-nm and 28-nm beads were 5.1% and 3.8% (within-run, n = 11), and 2.9% and 6.2% (between-run, n = 3), respectively. The lipoprotein sizes determined by DLS for lipoprotein fractions isolated by chromatography were consistent with the elution profile. Whole serum, four isolated lipoprotein fractions (CM + VLDL + IDL, large LDL, sd LDL, and HDL) and a non-lipoprotein fraction isolated by sequential ultracentrifugation were determined by DLS to be 13.1 ± 7.5 nm, 37.0 ± 5.2 nm, 21.5 ± 0.8 nm, 20.3 ± 1.1 nm, 8.6 ± 1.5 nm, and 8.8 ± 2.0 nm, respectively. Conclusions: The proposed DLS method can differentiate the sizes of isolated lipoprotein particles, including large LDL and sd LDL, and might be used in clinical laboratories in combination with convenient lipoprotein separation.

Published

2010