Plasma protein binding of (99m)Tc-labeled hydrazino nicotinamide derivatized polypeptides and peptides

M Ono; Y Arano; T Mukai; T Uehara; Y Fujioka; K Ogawa; S Namba; M Nakayama; T Saga; J Konishi; K Horiuchi; A Yokoyama; H Saji

doi:10.1016/s0969-8051(00)00200-6

Plasma protein binding of (99m)Tc-labeled hydrazino nicotinamide derivatized polypeptides and peptides

Nucl Med Biol. 2001 Feb;28(2):155-64. doi: 10.1016/s0969-8051(00)00200-6.

Authors

M Ono¹, Y Arano, T Mukai, T Uehara, Y Fujioka, K Ogawa, S Namba, M Nakayama, T Saga, J Konishi, K Horiuchi, A Yokoyama, H Saji

Affiliation

¹ Department of Patho-Functional Bioanalysis, Graduate School of Pharmaceutical Sciences, Kyoto University, Yoshida-shimoadachi-cho, Sakyo-ku, Kyoto 606-8501, Japan.

PMID: 11295426
DOI: 10.1016/s0969-8051(00)00200-6

Abstract

6-Hydrazinopyridine-3-carboxylic acid (HYNIC) constitutes one of the most attractive reagents to prepare (99m)Tc-labeled polypeptides and peptides of various molecular weights in combination with two tricine molecules as coligands. Indeed, (99m)Tc-HYNIC-conjugated IgG showed biodistribution of radioactivity similar to that of (111)In-DTPA-conjugated IgG. However, recent studies indicated significant plasma protein binding when the (99m)Tc labeling procedure was expanded to low molecular weight peptides. In this study, pharmacokinetics of (99m)Tc-HYNIC-conjugated IgG, Fab and RC160 using tricine were compared with their radioiodinated counterparts to evaluate this (99m)Tc-labeling method. In mice, [(99m)Tc](HYNIC-IgG)(tricine)(2) and [(99m)Tc](HYNIC-Fab)(tricine)(2) showed persistent localization of radioactivity in tissues when compared with their (125)I-labeled counterparts. [(99m)Tc](HYNIC-IgG)(tricine)(2) eliminated from the blood at a rate similar to that of (125)I-labeled IgG, while [(99m)Tc](HYNIC-Fab)(tricine)(2) showed significantly slower clearance of the radioactivity than (125)I-labeled Fab. On size-exclusion HPLC analyses, little changes were observed in radiochromatograms after incubation of [(99m)Tc](HYNIC-IgG)(tricine)(2) in murine plasma. However, [(99m)Tc](HYNIC-Fab)(tricine)(2) and [(99m)Tc](HYNIC-RC160)(tricine)(2) demonstrated significant increases in the radioactivity in higher molecular weight fractions in plasma. Formation of higher molecular weight species was reduced when [(99m)Tc](HYNIC-RC160)(tricine)(2) was stabilized with nicotinic acid (NIC) to generate [(99m)Tc](HYNIC-RC160)(tricine)(NIC). [(99m)Tc](HYNIC-RC160)(tricine)(NIC) also demonstrated significantly faster clearance of the radioactivity from the blood than [(99m)Tc](HYNIC-RC160)(tricine)(2). These findings suggested that one of the tricine coligands in (99m)Tc-HYNIC-labeled (poly)peptides would be replaced with plasma proteins to generate higher molecular weight species that exhibit slow blood clearance. In addition, the molecular sizes of parental peptides played an important role in the progression of the exchange reaction of one of the tricine coligands with plasma proteins.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Blood Proteins / metabolism*
Immunoglobulin Fab Fragments
Immunoglobulin G / blood
Indium Radioisotopes / pharmacokinetics
Male
Mice
Mice, Inbred Strains
Organotechnetium Compounds / blood
Organotechnetium Compounds / chemical synthesis
Organotechnetium Compounds / pharmacokinetics*
Pentetic Acid / pharmacokinetics
Protein Binding
Radiopharmaceuticals / blood
Radiopharmaceuticals / chemical synthesis
Radiopharmaceuticals / pharmacokinetics*
Tissue Distribution

Substances

Blood Proteins
Immunoglobulin Fab Fragments
Immunoglobulin G
Indium Radioisotopes
Organotechnetium Compounds
Radiopharmaceuticals
technetium Tc 99m hydrazinonicotinate-IgG
Pentetic Acid