Your search keyword '"Chen BM"' showing total 7 results

1. Sensitivity of PEGylated interferon detection by anti-polyethylene glycol (PEG) antibodies depends on PEG length.

Author

Cheng TC, Chuang KH, Chen M, Wang HE, Tzou SC, Su YC, Chuang CH, Kao CH, Chen BM, Chang LS, Roffler SR, and Cheng TL

Subjects

Animals, Female, Humans, Interferons blood, Mice, Polyethylene Glycols pharmacokinetics, Antibodies immunology, Enzyme-Linked Immunosorbent Assay methods, Interferons analysis, Interferons chemistry, Polyethylene Glycols chemistry

Abstract

Attachment of poly(ethylene glycol) to proteins can mask immune epitopes to increase serum half-life, reduce immunogenicity, and enhance in vivo biological efficacy. However, PEGylation mediated epitope-masking may also limit sensitivity and accuracy of traditional ELISA. We previously described an anti-PEG-based sandwich ELISA for universal assay of PEGylated molecules. Here, we compared the quantitative assessment of PEGylated interferons by anti-PEG and traditional anti-interferon sandwich ELISA. The detection limits for PEG-Intron (12k-PEG) and Pegasys (40k-PEG) were 1.9 and 0.03 ng/mL for anti-PEG ELISA compared to 0.18 and 0.42 ng/mL for traditional anti-interferon sandwich ELISA. These results indicate that the anti-PEG sandwich ELISA was insensitive to PEGylation mediated epitope-masking and the sensitivity increased in proportion to the length of PEG. By contrast, PEG-masking interfered with detection by traditional anti-interferon sandwich ELISA. Human and mouse serum did not affect the sensitivity of anti-PEG ELISA but impeded traditional anti-interferon sandwich ELISA. The anti-PEG sandwich ELISA was comparable to anti-interferon sandwich ELISA and radioassay of 131I-Pegasys in pharmacokinetic studies in mice. The anti-PEG sandwich ELISA provides a sensitive, accurate, and convenient quantitative measurement of PEGylated protein drugs.

Published

2013

2. Analytical measurement of PEGylated molecules.

Author

Cheng TL, Chuang KH, Chen BM, and Roffler SR

Subjects

Animals, Chromatography, High Pressure Liquid methods, Colorimetry methods, Enzyme-Linked Immunosorbent Assay methods, Humans, Isotope Labeling methods, Liposomes chemistry, Pharmaceutical Preparations chemistry, Polyethylene Glycols pharmacokinetics, Proteins chemistry, Polyethylene Glycols analysis

Abstract

Attachment of poly(ethylene glycol) (PEG) to proteins, peptides, liposomes, drugs, and nanoparticles can improve pharmaceutical pharmacokinetic properties and enhance in vivo biological efficacy. Since the first PEGylated product was approved by the Food and Drug Administration in 1990, increasing numbers of PEGylated compounds have entered clinical use. Successful clinical development of PEGylated pharmaceuticals requires accurate methods for the qualitative and quantitative analysis of intact PEG conjugates in biological fluids. In this article, we review assay methods that can be utilized for the detection and measurement of PEGylated pharmaceuticals in complex biological samples for determination of biodistribution and pharmacokinetic properties. In particular, we describe relevant colorimetric, chromatographic, radiolabeled, biological, and enzyme-linked immunosorbent assays for the pharmacokinetic study of PEGylated molecules.

Published

2012

3. A humanized immunoenzyme with enhanced activity for glucuronide prodrug activation in the tumor microenvironment.

Author

Chen KC, Wu SY, Leu YL, Prijovich ZM, Chen BM, Wang HE, Cheng TL, and Roffler SR

Subjects

Animals, Antibodies, Neoplasm chemistry, Antibodies, Neoplasm isolation & purification, Antineoplastic Agents metabolism, Antineoplastic Agents pharmacology, Biocatalysis, Cell Line, Tumor, Cell Proliferation drug effects, Dose-Response Relationship, Drug, Glucuronidase chemistry, Glucuronidase isolation & purification, Glucuronides pharmacology, Humans, Mice, Mice, Inbred BALB C, Mice, Nude, Mice, SCID, Molecular Imaging, NIH 3T3 Cells, Prodrugs pharmacology, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins isolation & purification, Structure-Activity Relationship, Xenograft Model Antitumor Assays, Antibodies, Neoplasm metabolism, Glucuronidase metabolism, Glucuronides metabolism, Prodrugs metabolism, Recombinant Fusion Proteins metabolism, Tumor Microenvironment

Abstract

Antibody-directed enzyme prodrug therapy (ADEPT) utilizing β-glucuronidase is a promising method to enhance the therapeutic index of cancer chemotherapy. In this approach, an immunoenzyme (antibody-β-glucuronidase fusion protein) is employed to selectively activate anticancer glucuronide prodrugs in the tumor microenvironment. A major roadblock to the clinical translation of this therapeutic strategy, however, is the low enzymatic activity and strong immunogenicity of the current generation of immunoenzymes. To overcome this problem, we fused a humanized single-chain antibody (scFv) of mAb CC49 to S2, a human β-glucuronidase (hβG) variant that displays enhanced catalytic activity for prodrug hydrolysis. Here, we show that hcc49-S2 displayed 100-fold greater binding avidity than hcc49 scFv, possessed greater enzymatic activity than wild-type hβG, and more effectively killed antigen-positive cancer cells exposed to an anticancer glucuronide prodrug as compared to an analogous hβG immunoenzyme. Treatment of tumor-bearing mice with hcc49-S2 followed by prodrug significantly delayed tumor growth as compared to hcc49-hβG. Our study shows that hcc49-S2 is a promising targeted enzyme for cancer treatment and demonstrates that enhancement of human enzyme catalytic activity is a powerful approach to improve immunoenzyme efficacy.

Published

2011

4. Sensitive quantification of PEGylated compounds by second-generation anti-poly(ethylene glycol) monoclonal antibodies.

Author

Su YC, Chen BM, Chuang KH, Cheng TL, and Roffler SR

Subjects

Animals, Antigen-Antibody Reactions, Enzyme-Linked Immunosorbent Assay, Mice, Mice, Inbred BALB C, Polyethylene Glycols chemistry, Proteins immunology, Antibodies, Monoclonal analysis, Antibodies, Monoclonal immunology, Polyethylene Glycols analysis, Proteins analysis, Proteins chemistry

Abstract

Poly(ethylene glycol) (PEG) is often attached to compounds to increase serum half-life, reduce immunogenicity, and enhance bioavailability. Accurate and sensitive quantification of PEG conjugates is critical for product development, pharmacokinetic measurements, and efficacy studies. However, PEGylated compounds can be difficult to quantify due to epitope masking by PEG. We previously generated two monoclonal antibodies to PEG (AGP3, IgM and E11, IgG) for quantitative detection of PEGylated proteins. We now report the identification of two second-generation mAbs to PEG (AGP4, IgM and 3.3, IgG) that bind to the repeating subunits of the PEG backbone and facilitate more sensitive quantification of a wider range of PEGylated compounds. A sandwich ELISA in which AGP4/3.3-biotin was employed as the capture/detection antibodies allowed quantification of PEG-Qdot 525 with 14-50-fold greater sensitivity than the original AGP3/E11 combination. Pegasys (PEG-interferon alpha-2a), PEG-Intron (PEG-interferon alpha-2b), Neulasta (PEG-G-CSF), and Lipo-Dox (PEGylated liposomal doxorubicin) could also be quantified with low ng/mL detection limits. The assay tolerated the presence of 50% human serum or 20% free PEG molecules. These new anti-PEG antibodies appear useful for qualitative and quantitative analysis of a wide range of PEGylated compounds.

Published

2010

5. Combination cancer therapy by hapten-targeted prodrug-activating enzymes and cytokines.

Author

Chuang KH, Cheng CM, Roffler SR, Lu YL, Lin SR, Wang JY, Tzou WS, Su YC, Chen BM, and Cheng TL

Subjects

Animals, Antibodies immunology, Antineoplastic Agents chemistry, Cell Line, Tumor, Drug Therapy, Combination, Glucuronidase chemistry, Glucuronidase metabolism, Interleukin-2 chemistry, Mice, Mice, Inbred BALB C, Neoplasms pathology, Polyethylene Glycols chemistry, Prodrugs pharmacology, Prodrugs therapeutic use, Antineoplastic Agents pharmacology, Glucuronidase pharmacology, Haptens immunology, Interleukin-2 pharmacology, Neoplasms drug therapy, Neoplasms immunology, Prodrugs metabolism

Abstract

Combination therapy can help overcome limitations in the treatment of heterogeneous tumors. In the current study, we examined whether multiple therapeutic agents could be targeted to anti-dansyl single-chain antibodies (DNS scFv) that were anchored on the plasma membrane of cancer cells. Functional DNS scFv could be stably expressed on CT-26 colon cancer cells both in vitro and in vivo. Dansyl moieties were covalently attached to recombinant beta-glucuronidase (betaG) and interleukin 2 (IL-2) via a flexible poly(ethylene glycol) linker to form DNS-PEG-betaG and DNS-PEG-IL-2 conjugates. The conjugates displayed enzymatic and splenocyte-stimulatory activities, respectively, that were similar to those of the unmodified proteins. The conjugates selectively bound CT-26 cells that expressed anti-DNS scFv (CT-26/DNS cells) but not CT-26 cells that expressed control scFv (CT-26/phOx cells). DNS-PEG-betaG preferentially activated a glucuronide prodrug (BHAMG) of p-hydroxy aniline mustard at CT-26/DNS cells in culture and accumulated in subcutaneous CT-26/DNS tumors after intravenous administration. Systemic administration of DNS-PEG-IL-2 or DNS-PEG-betaG and BHAMG significantly delayed the growth of CT-26/DNS but not control CT-26/phOx tumors. Combination treatment with DNS-PEG-betaG and BHAMG followed by DNS-PEG-IL-2 therapy significantly suppressed the growth of CT-26/DNS tumors as compared to either single-agent regimen. These results show that at least two DNS-modified therapeutic agents can be selectively delivered to DNS scFv receptors in vitro and in vivo, allowing combination therapy of DNS scFv-modified tumors.

Published

2006

6. Monoclonal antibody-based quantitation of poly(ethylene glycol)-derivatized proteins, liposomes, and nanoparticles.

Author

Cheng TL, Cheng CM, Chen BM, Tsao DA, Chuang KH, Hsiao SW, Lin YH, and Roffler SR

Subjects

Animals, Cell Line, Tumor, Enzyme-Linked Immunosorbent Assay, Female, Liposomes immunology, Mice, Proteins immunology, Antibodies, Monoclonal immunology, Liposomes analysis, Liposomes chemistry, Nanostructures analysis, Polyethylene Glycols chemistry, Proteins analysis, Proteins chemistry

Abstract

Covalent attachment of poly(ethylene glycol) (PEG) molecules to drugs, proteins, and liposomes is a proven technology for improving their bioavailability, safety, and efficacy. Qualitative and quantitative analysis of PEG-derivatized molecules is important for both drug development and clinical applications. We previously reported the development of a monoclonal IgM antibody (AGP3) to PEG. We now describe a new IgG1 monoclonal antibody (E11) to PEG and show that it can be used in combination with AGP3 to detect and quantify PEG-derivatized molecules. Both antibodies bound the repeating subunits of the PEG backbone and could detect free PEG and PEG-modified proteins by ELISA, immunoblotting, and flow cytometry. Detection sensitivity increased with the length and the number of PEG chains on pegylated molecules. Both antibodies also efficiently accelerated the clearance of a PEG-modified enzyme in vivo. A sandwich ELISA in which E11/AGP3 were employed as the capture/detection antibodies was developed to detect PEG-modified proteins at concentrations as low as 1.2 ng/mL. In addition, the ELISA could also quantify, in the presence of 10% fetal bovine serum, free methoxy-PEG20,000, PEG2,000-quantum dots, and PEG2,000-liposomes at concentrations as low as 20 ng/mL (1.0 nM), 1.4 ng/mL (3.1 pM), and 2.4 ng/mL (3.13 nM phospholipids), respectively. Finally, we show that the sandwich ELISA could accurately measured the in vivo half-life of a PEG-modified enzyme. These antibodies should be generally applicable to the qualitative and quantitative analysis of all PEG-derivatized molecules.

Published

2005

7. Efficient clearance of poly(ethylene glycol)-modified immunoenzyme with anti-PEG monoclonal antibody for prodrug cancer therapy.

Author

Cheng TL, Chen BM, Chern JW, Wu MF, and Roffler SR

Subjects

Aniline Mustard analogs & derivatives, Aniline Mustard chemistry, Aniline Mustard therapeutic use, Aniline Mustard toxicity, Animals, Antibodies, Monoclonal chemistry, Antibodies, Monoclonal therapeutic use, Antineoplastic Agents chemistry, Antineoplastic Agents toxicity, Cell Survival drug effects, Disease Models, Animal, Drug Carriers chemistry, Drug Carriers pharmacokinetics, Escherichia coli enzymology, Glucuronidase chemistry, Glucuronidase immunology, Humans, Immunoenzyme Techniques methods, Immunoglobulin Fab Fragments chemistry, Iodine Radioisotopes, Mice, Mice, Inbred BALB C, Mice, Nude, Neoplasm Transplantation, Polyethylene Glycols chemistry, Prodrugs chemistry, Prodrugs therapeutic use, Tissue Distribution, Transplantation, Heterologous, Tumor Cells, Cultured, Antibodies, Monoclonal pharmacokinetics, Antineoplastic Agents therapeutic use, Glucuronidase pharmacokinetics, Polyethylene Glycols pharmacokinetics, Prodrugs pharmacokinetics

Abstract

The F(ab')(2) fragment of the anti-TAG-72 antibody, B72.3, was covalently linked to Escherichia coli-derived beta-glucuronidase that was modified with methoxypoly(ethylene glycol). The conjugate (B72.3-betaG-PEG) localized to a peak concentration in LS174T xenografts within 48 h after injection, but enzyme activity persisted in plasma such that prodrug administration had to be delayed for at least 4 days to avoid systemic prodrug activation and associated toxicity. Conjugate levels in tumors decreased to 36% of peak levels at this time. Intravenous administration of AGP3, an IgM mAb against methoxypoly(ethylene glycol), accelerated clearance of conjugate from serum and increased the tumor/blood ratio of B72. 3-betaG-PEG from 3.9 to 29.6 without significantly decreasing the accumulation of conjugate in tumors. Treatment of nude mice bearing established human colon adenocarcinoma xenografts with B72. 3-betaG-PEG followed 48 h later with AGP3 and a glucuronide prodrug of p-hydroxyaniline mustard significantly (p< or =0.0005) delayed tumor growth with minimal toxicity compared to therapy with a control conjugate or conventional chemotherapy.

Published

2000