Studies on the preparation of186ReDTPA complexes using low specific activity186Re for antibody labeling

¹⁸⁶Re is considered as Therapy Isotope and can be used in radioimmunotherapy. The radiation characteristics of this isotope are ideal for therapy. Generally metallic radionuclides are labeled to antibodies through bifunctional chelating agents, such as DTPA (diethylenetetraaminepentaacetic acid). A study has been carried out on the complexation of DTPA with¹⁸⁶Re using low specific activity¹⁸⁶Re. This was carried out to evaluate various parameters which are involved in the complex formation including methods of processing of raw material¹⁸⁶Re. Stannous chloride was used as the reducing agent for the reduction of rhenium. Different labeling conditions such as pH, time, temperature and concentration of reducing agent were all studied for complex formation. The complex was characterized by paper electrophoresis, paper chromatography and gel column chromatography.     

A new technique for labeling of Lipiodol with 188Re in the treatment of hepatic tumor

A new method for the synthesis of ¹⁸⁸Re-Lipiodol without using a chelating agent and to evaluate the stability and biodistribution of the new agent in rats with hepatic tumors was attempted. Eighteen male Sprague -Dawley rats with liver tumors were sacrificed at 1, 24, and 48 hours (six rats at each time) after injection of approximately 7.4 MBq (0.2 mCi) of ¹⁸⁸Re Lipiodol via the hepatic artery. Samples of tumor, liver and other organs were collected and tissue concentration (%ID/g) of the markers were calculated. Our data showed a high level of radioactivity in the hepatic tumors at every time of the study. The ratios of tumor to normal liver tissue concentration (T/N ratio) were 7.62 at 1 hour, 8.03 at 24 hours, and 7.70 at 48 hours. Except for the liver, kidneys and lungs, concentrations in other organs were low. The new method for labeling Lipiodol with ¹⁸⁸Re is simple and has potential for the treatment of hepatic tumors This revised version was published online in July 2006 with corrections to the Cover Date.     

A study on photolinkers used for biomolecule attachment to polymer surfaces

The use of photolinkers (photoactivatable heterobifunctional crosslinkers) is a popular method to attach biomolecules to polymer surfaces. This study addresses the selection of photolinker and the adjustment of reaction conditions, such as the concentration of biomolecule applied, and irradiation time. The influence of these variables are investigated for four prominent photolinkers: ketyl-reactive benzophenone (BP) and anthraquinone (AQ), nitrene-reactive nitrophenyl azide (NPA), and carbene-reactive phenyl-(trifluoromethyl)diazirine (PTD). The influence of substrate material is discussed, and three different polymers served as representative substrates: poly(methyl methacrylate) (PMMA), polystyrene (PS), and a cycloolefin copolymer (COC). We compared the overall photolinking efficiency of all photolinkers with respect to the polymer substrate they are applied to, and we found considerable differences for certain photolinker/substrate combinations. Of all photolinkers and substrates tested, PTD as photolinker and COC as substrate showed the highest photolinking efficiencies and fastest reaction times. For this study DNA oligonucleotides were chosen as a model system of biomolecular probes, and fluorescence detection of DNA microarrays served as method of detection.     

Peptide labeling using 188Re, 188Re-MAG3 and 153Sm-H1ETA: A comparison on their in vitro lipophilicity

Lanreotide peptide was labeled with ¹⁵³Sm-H₁ETA and ¹⁸⁸Re-MAG₃ in order to evaluate whether or not their conjugation to the peptide produce significant differences of the in vitro lipophilicity with respect to the ¹⁸⁸Re-lanreotide prepared by the direct labeling method (highly lipophilic). The differences of lipophilicity between the complexes, were evaluated using a reverse phase HPLC system. The measured lipophilicity of ¹⁵³Sm-H₁ETA-lanreotide, ¹⁸⁸Re-MAG₃-lanreotide and ¹⁸⁸Re-lanreotide was taken to be the capacity factor [k" = (t _R-t ₀)/t ₀ where t _R is the retention time and t ₀ is the dead time] for each of the complexes under identical chromatography conditions. Results showed that the in vitro lipophilicity decreased in the order ¹⁸⁸Re-lanreotide (direct labeling), ¹⁸⁸Re-MAG₃-lanreotide and ¹⁵³Sm-H₁ETA-lanreotide. Since the last one has a capacity factor (k") similar to that of ¹⁸⁸Re-MAG₃, some renal elimination for ¹⁵³Sm-H₁ETA-lanreotide could be expected, which probably would reduce the unnecessary radiation dose to normal tissues.     

An improved synthesis of S-benzoyl mercaptoacetyltriglycine as BFCA and the labeling of IgG with carrier-free 188Re

S-benzoyl mercaptoacetyltriglycine (S-Bz-MAG₃) was synthesized and labeled with carrier-free ¹⁸⁸Re. The overall yield of S-Bz-MAG₃ is higher than those published in the literature. Dependence of the labeling yield of ¹⁸⁸Re-MAG₃ upon concentration of reducing agent, pH, reaction time, and other parameters was examined and optimum conditions were obtained. The labeling yield of ¹⁸⁸Re-MAG₃ was more than 98%. The concentration procedure was succeeded with Sep-Pak C18 column to obtain highly concentrated ¹⁸⁸Re-MAG₃. The experimental conditions of labeling of IgG with carrier free ¹⁸⁸Re via S-Bz-MAG₃ as a bifunctional chelating agent (BFCA) by pre-radiolabeling of the chelate was studied. The conjugation conditions were optimized. The stability of ¹⁸⁸Re-MAG₃-IgG in vitro was high. The results of this studiy may be useful for ¹⁸⁸Re labeling of MAbs for radioimmunotherapy.     

Extrapolation equations for determining solubility activity products for dilute solutions of perchlorates and perrhenates

Extrapolation equations derived from activity coefficient expressions which account for specific interactions of ions, including an adaptation of Pitzer's equation, are used in the determination of solubility (activity) products for some perchlorates and perrhenates. Solubility data at 25°C on the molarity (mol-dm^–3) scale are used. A comparison of the results obtained with different extrapolation equations is made in order to determine the most appropriate one to use.     

Analysis of beryllium to biomolecule binding using a metal specific fluorescent probe and competitive assay

Studying metal-biomolecule interactions is critical to the elucidation of the molecular basis of the biological functions and toxicity of metals. In the present study, a competitive fluorimetric approach has been developed to measure the apparent affinity of biomolecules for Be²⁺ by using a Be²⁺-specific fluorigenic probe (10-hydroxybenzo[h]quinoline-7-sulfonate, HBQS). Under physiological conditions, HBQS coordinates with Be²⁺ in a molar ratio of 1:1 and results in a fluorescence shift from 580 nm for HBQS to 480 nm for the Be-HBQS complex associated with significant fluorescence enhancement. When a beryllium ligand is present in the mixture of Be²⁺ and HBQS, the competition of ligand against HBQS for beryllium ion binding results in dissociation and thus a fluorescence decrease of the Be-HBQS complex. By titrating ligand and monitoring the dose-dependent decrease of Be-HBQS complex fluorescence at 480 nm, the apparent affinity between ligand and Be²⁺ can be derived. Applying this simple approach, the apparent affinities of various nucleotides and the iron-storage protein ferritin for beryllium ion have been determined. In particular, the apparent dissociation constant of Be²⁺ and adenosine 5′-triphosphate (ATP) was also validated by an electrospray ionization mass spectrometric (ESI-MS) method. The general applicability of the proposed competition assay was further demonstrated using FluoZin-1, a zinc fluorescent indicator, in a binding study for Zn²⁺ and bovine serum albumin. This newly developed competitive fluorimetric assay provides a sensitive, simple, and generic approach for affinity estimation of metal and biomolecule binding.     

Production study of high specific activity NCA Re-186g by proton and deuteron cyclotron irradiation

Very high specific activity (A_S) ^186gRe could be produced by either proton or deuteron cyclotron irradiation on highly enriched ¹⁸⁶W target in no-carrier-added (NCA) form, leading to a A_S very close to the theoretical carrier free (CF) value of 6.88 GBq μg⁻¹. Thick Target Yields (TTYs), obtained irradiating both thick metal W targets of natural isotopic composition and highly enriched powdered ¹⁸⁶W targets, were measured at different particles energies taking into account high accuracy and precision. The evaluation of radionuclidic purities of ^186gRe obtained activating highly enriched ¹⁸⁶W by both p and d were also carried out and accurately compared. The thin-target excitation functions for all Re (A = 181, 182, 183, 184, 186 and their metastable levels), and W and Ta coproduced radionuclides will be presented elsewhere in deep details.     

Solvent Extraction of Rhenium(VII) for Preparation of No-Carrier-Added 186Re Saline Solution with High Specific Volume Activity

By using ¹⁸⁸Re as a radiotracer, the extraction behavior of Re(VII) by a tertiary amine extractant N-235 from HCl and the back-extraction behavior of Re(VII) by HNO₃ and ammonia were studied. A chemical separation procedure, which combined the acid alumina column and solvent extraction was established. The procedure was rapid and efficient for the separation of ¹⁸⁶Re from ¹⁸⁶W irradiated by 16 MeV deuterons. No-carrier-added ¹⁸⁶ReO₄ ^– saline solution with high specific volume activity was obtained. The overall recovery yield of ¹⁸⁶Re was about 85%.     

The hydrazide/hydrazone click reaction as a biomolecule labeling strategy for M(CO)3 (M = Re, (99m)Tc) radiopharmaceuticals

Facile reactivity of hydrazides and aldehydes was explored as potential coupling partners for incorporation into M(CO)(3) (M = Re, (99m)Tc) based radiopharmaceuticals. Both 'click, then chelate' and 'prelabel, then click' synthetic routes produced identical products in high yields and lacked metal-hydrazide/-hydrazone interactions, highlighting the potential of this click strategy.     

Selected reaction monitoring (SRM) mass spectrometry without isotope labeling can be used for rapid protein quantification

The validation of putative biomarker candidates has become the major bottle-neck in protein biomarker development. Conventional immunoaffinity methods are limited by the availability of antibodies and kits. Here we demonstrate the feasibility of using selected reaction monitoring (SRM) without isotope labeling to achieve fast and reproducible quantification of serum proteins. The SRM/MRM assays for three standard serum proteins, including ceruloplasmin (CP), serum aymloid A (SAA) and sex hormone binding globulin (SHBG), have good linear ranges, generally 10(3) to 10(4) . There are almost perfect correlations between SRM intensities and the loaded peptide amounts (R(2) is usually ~0.99). Our data suggest that SRM/MRM is able to quantify proteins within the range of 0.2-2 fmol, which is comparable to the commercial ELISA/LUMINEX kits for these proteins. Excellent correlations between SRM/MRM and ELISA/LUMINEX assays were observed for SAA and SHBG (R(2)=0.928 and 0.851, respectively). However, the correlation between SRM/MRM and ELISA for CP is less desirable (R(2)=0.565). The reproducibility for SRM/MRM assays is generally very good but may depend on the proteins/peptides being analyzed (R(2)=0.931 and 0.882 for SAA and SHBG, and 0.723 for CP). The SRM/MRM assay without isotope labeling is a rapid and useful method for protein biomarker validation in a modest number of samples and is especially useful when other assays such as ELISA or LUMINEX are not available.     

Synthesis and characterization of dimaleimide fluorogens designed for specific labeling of proteins

A series of aromatic compounds were prepared bearing two maleimide groups attached directly to the fluorescent cores. The resulting derivatives do not fluoresce until the maleimide groups undergo their typical thiol addition reaction, thus removing their ability to quench fluorescence, as shown by kinetic and spectral characterization studies. In this way, the title compounds serve as fluorogens capable of detection of small thiols or appropriately sized dithiols. Recombinant alpha-helical proteins were then designed to bear two cysteine residues capable of regioselective dithiol addition reaction with the dimaleimide fluorogens, thus acting as spatially encoded substrates that form specifically labeled covalent complexes. The efficiency of this in vitro fluorescent protein-labeling reaction demonstrates the feasibility of the development of a method for the fluorescent labeling of specific recombinant proteins.     

A simple method for the determination of the specific activity of125I-tracer used in radioimmunoassay

Knowledge of the specific activity of the¹²⁵I-tracer is essential for optimization and for calculation of RIA parameters. The specific activity of the¹²⁵I-thyroxin used in thyroxin radioimmunoassay /RIA/ has been determined by a simple method involving combination of RIA and displacement analysis. It has been compared with the value obtained by the conventional method based on radioiodination data. Our studies indicate that even for a non-protein hormone like thyroxin the specific activity of¹²⁵I-thyroxin derived from iodination data is not reliable. The specific activities obtained by displacement analysis were consistent with the experimental findings.     

Synthesis of amino-modified magnetite nanoparticles coated with Hepama-1 and radiolabeled with 188Re for bio-magnetically targeted radiotherapy

Summary  Elérh     

High specific activity carbon-11 labelling of benzodiazepines: Diazepam and flunitrazepam

In order to study “in vivo” the brain specific receptor sites of benzodiazepines, a method for carbon-11 labelling of diazepam and flunitrazepam without irradiation risk to personnel is described. 70 mCi (max. 140 mCi) of injectable labelled product, chemically and radiochemically pure, are obtained in 45 minutes with a specific activity of 810 Ci/m mole.     

Synthesis and functionalization of carbon xerogels to be used as supports for fuel cell catalysts

The synthesis and properties of carbon xerogels are briefly described in this mini-review, emphasizing the methods used for tuning their surface chemistry and textural properties in order to design efficient electrocatalysts for fuel cells. In particular, the role played by the surface functional groups in determining the loading, dispersion, oxidation state and stability of the metal phases is addressed.     

A glucosamine-dipicolylamine conjugate of 99mTc(I) and 186Re(I) for use in imaging and therapy

The synthesis and metal complexation of a glucosamine-appended 2,2'-dipicolylamine ligand to the tricarbonyls of 99mTc and 186Re is described; the ligand was found to bind in a tridentate fashion with the glucosamine function remaining pendant, and the 99mTc complex was found to exhibit exceptional stability towards in vitro ligand exchange experiments.     

A light detection cell to be used in a micro analysis system for ammonia

This paper describes the design, realization and characterization of a micromachined light detection cell. This light detection cell is designed to meet the specifications needed for a micro total analysis system in which ammonia is converted to indophenol blue. The concentration of indophenol blue is measured in a light detection cell. The light detection cell was created using KOH/IPA etching of silicon. The KOH/IPA etchant was a 31 wt.% potassium hydroxide (KOH) solution with 250 ml isopropyl alcohol (IPA) per 1000 ml H(2)O added to it. The temperature of the solution was 50 degrees C. Etching with KOH/IPA results in 45 degrees sidewalls ({110} planes) which can be used for the in- and outcoupling of the light. The internal volume of the realized light detection cell is smaller than 1 mul, enabling measurements on samples in the order of only 1 mul. Measurements were performed on indophenol blue samples in the range of 0.02 to 50 muM. In this range the measurements showed good reproducibility.