Enhanced rectal absorption of amphotericin B lyophilized with glycyrrhizinate in rabbits

The influence of bases and additives in the formulation for rectal absorption of amphotericin B (AMB) lyophilized with dipotassium glycyrrhizinate (GLYK) was investigated using rabbits in relation to an in vitro release test. The release of AMB from the fatty base of Witepsol or a medium chain triglyceride (MCT) was markedly faster than that from the hydrophilic base of macrogol. The addition of polyoxyethylene (2) lauryl ether (POE(2)LE) into the fatty bases led to a marked increase in the release rate, whereas POE(9)LE or sodium lauryl sulfate resulted in a significantly lower release rate. Animals received rectally each of seven AMB formulations of Witepsol H-15, macrogol, MCT with surfactants and aqueous solution. The absorption of the AMB lyophilized mixture with GLYK at a 1:9 molar ratio from a MCT base was significantly superior to that from macrogol. The addition of POE(2)LE into the MCT base resulted in a marked increase in bioavailability, showing the highest bioavailability of 4.9%. High serum levels of over 100 ng/ml of serum were maintained for 24 h following administration. The lowest bioavailability was 0.32% for the macrogol suppository. There was a good correlation between the release rate of AMB from the formulations and bioavailability. These results suggest that an AMB rectal formulation may provide a promising therapeutic alternative to infusion, taking into account the serum level of AMB exceeding the minimal inhibitory concentration of the infecting organism.     

A simple technique for reconstruction of the umbilicus, using two twisted flaps

A successful umbilical reconstruction is described, using two twisted flaps with one pedicle. This technique is easy and simultaneously revises the scar of the abdominal wall. With this procedure, the umbilicus has a natural appearance with sufficient depression and normal-appearing wrinkles.     

Prevention of bone loss by percutaneous estradiol implants in ovariectomized rats

This study was conducted to investigate whether hydroxyapatite (HAP) is appropriate as a percutaneous drug carrier for estradiol (E2) for the suppression of bone loss. Ten-week-old female Sprague-Dawley rats were subjected either to bilateral ovariectomy (OVX) or to sham surgery (control). Ovariectomized rats were implanted percutaneously with E2-HAP disks containing low, medium or high doses of estradiol (50, 250, or 500 micrograms E2/rat, respectively). Ovariectomized rats without implant and OVX rats implanted only with HAP served as additional controls. All rats were sacrificed 90 days after surgery. At the end of the experiment, bone mineral density of the lumbar spine was measured by dual energy X-ray absorption, and serum E2 was assayed by radioimmunoassay. The bone mineral density of OVX and HAP-treated OVX rats decreased by 18% compared to sham surgery rats, but decreased by only 13, 7, and 3% in rats treated with 50, 250, and 500 micrograms E2/rat, respectively. The in vitro release of E2 from E2-HAP devices was determined by an HPLC method. Estradiol release from the HAP devices followed almost a zero-order kinetics. Estradiol remained intact in E2-HAP implants for up to six months when stored at 5, 25, and 40 degrees C. This study indicates that E2-HAP implants are effective in suppressing bone loss in the spine of OVX rats in a dose-dependent manner.     

Astrocytic contributions to blood-brain barrier (BBB) formation by endothelial cells: a possible use of aortic endothelial cell for in vitro BBB model

Astrocytic contribution of endothelial cell monolayer permeability was examined in two blood-brain barrier (BBB) models, using the coculture in a double chamber system: rat astrocytes and bovine aortic endothelial cells (BAECs) or bovine brain endothelial cells (BBECs). In system 1, where astrocytes were separated from endothelial cells, a 40% reduction in L-glucose permeability of the BBEC monolayer, but not the BAEC monolayer, was observed by cocultivation with astrocytes. Although several passages of BBEC in culture elicited morphological transformation from spindle-shapes to cobblestone-like features, the passaged BBECs remained responsive to astrocytes in coculture in system 1 (37% reduction of the L-glucose permeability). By contrast, in system 2, where respective endothelial cells and astrocytes layered on the upper and lower surfaces of a membrane, the permeability of both BAEC and BBEC monolayers was reduced by cocultivation with astrocytes (75% reduction for BAEC and 40% reduction for BBEC). BAECs in this contiguous coculture (system 2) with astrocytes showed numerous tight junction-like structures characteristic of the BBB in vivo. These results suggest that primary cultured BBECs, which had been primed by astrocytes in vivo, retain a higher sensitivity to astrocytes possibly through an astrocytic soluble factor (s) to exhibit BBB-specific phenotypes, and that even BAEC from extra-neural tissues, when cultured with astrocytes in close proximity in vitro, may acquire the similar phenotypes and serve for an extensive use of BBB model in vitro.     

Application of alginate gel as a vehicle for liposomes. II. Erosion of alginate gel beads and the release of loaded liposomes

Short chain fatty acids (SCFAs) stimulate electroneutral sodium absorption by activation of apical Na/H exchange in colonocytes. It is often assumed that activation of Na/H exchange is via an intracellular acidification caused by SCFA uptake. These lecture notes review shortcomings in this model of SCFA-stimulated sodium absorption, revealed by recent reports in the literature. This is supplemented by information generated in our laboratory using both a tissue culture model of colonocytes (HT29-C1 cells) and a native tissue preparation (mouse distal colonic mucosa). In both preparations, evidence suggests that physiologic SCFA gradients may generate pH heterogeneity in aqueous microdomains near the plasma membrane of colonocytes. Finally, direct observation of such extracellular microdomains with confocal microscopy is used to support a new model, in which pH microdomains play an important role in regulating both SCFA fluxes and sodium absorption.     

Complexation of Be(II) Ion with 1-(2,4-Dihydroxy-1-phenylazo)-8-hydroxy-3,6-naphthalenedisulfonate as the Chemical Basis of the Selective Detection of Ultratrace Be by Reversed-Phase High-Performance Liquid Chromatography

The complexation reactions of beryllium(II) ion with 1-(2,4-dihydroxy-1-phenylazo)-8-hydroxy-3,6-naphthalenedisulfonate (H-resorcinol) are studied. The acid dissociation constants of H-resorcinol, H(3)L(2-), at 293 K and I = 0.10 [K(OH, NO(3))] are pK(a)((1)) = 5.67, pK(a)((2)) = 8.57, and pK(a)((3)) > 13. The formation constant at 293 K and I = 0.10 [(K,H)NO(3)] is estimated to be log[{[Be(HL)(2-)][H(+)](2)}/{[Be][H(3)L(2-)]}] = -4.58, and pK(a)' = 6.39 for [Be(HL)](2-), which give the basis for the optimization of the precolumn chelation reactions and the masking system with EDTA. The kinetic data for ligand substitution reactions with sulfosalicylate ion are also reported to demonstrate the remarkable inertness of the Be chelate, which is suitable for HPLC separation. Reported is an accurate method for determining traces of Be(II) ion at nanomolar levels with photometric detection coupled with ion-pair reversed-phase HPLC. The chelate, [Be(II)L](3-), is efficiently separated on an Asahipak ODP-50 column using tetrabutylammonium bromide as an ion-pairing agent in a methanol (35 wt %)-water eluent. Only Al and Fe give peaks under the conditions used. The large molar absorptivity of the H-resorcinol chelate, 3.99 × 10(4) M(-1) cm(-1) at 500 nm, and the short retention time with excellent peak resolution ensure the ultralow detection limit (3σ blank) down to 7.2 ppt (0.8 nM) with no preconcentration procedures. The excellent toughness toward the matrix influence was demonstrated using the model solution for an air-dust sample. The HPLC separation, coupled with the EDTA masking procedure, enables one to detect Be(II) ion at 20 nM in the presence of metals at the natural abundance levels in air samples, such as Al, Fe, Ca, Mg, Zn, and Pb at 240, 140, 300, 66, 16, and 6.2 μM, respectively, in the final solution.     

Possibility of alpha-tricalcium phosphate (alpha-TCP) particles as a drug carrier for treatment of abdominal carcinomatosis

It is reported that cancer foci are unevenly distributed in abdominal carcinomatosis after intraperitoneal inoculation of cancer cells in rats. The organs may be briefly classified into two groups in terms of the deposit of cancer cells: one that shows an affinity to the cells includes the greater omentum, mesenterium, and gonadal fat and etc., and the other having lesser affinity the stomach, intestine, and spleen and etc. Such uneven distributions are likely to occur in clinical cases of abdominal carcinomatosis resulting from progressive digestive cancers. We have explored the possibility of alpha-Tricalcium Phosphate (alpha-TCP) particles as a drug carrier in which carboplatin (CBDCA) was incorporated. alpha-TCP, which has chemically similar properties to hydroxyapatite, is known to have an excellent biocompatibility with human tissues and is biodegradable. The present study focused on the localization and the forms of alpha-TCP particles, and the morphological changes of the surrounding tissues after intraperitoneal administration using normal and cancer-bearing rats. The following results were obtained: (1) alpha-TCP particles were taken up to a large extent in the "milky spot" of the greater omentum, followed by the "stomata" of the mesenterium, gonadal fat, diaphragm, peritoneum, and liver in normal rats. No alpha-TCP particles were caught up in the tissues of the stomach, small intestine, colon, and spleen. The margination and emigration of lymphocytes were slightly observed around those organs. (2) alpha-TCP particles were predominantly detected on the cancer mass of the greater omentum in abdominal carcinomatosis-bearing rats. It should be noted that the particles collected in the same place where cancer cells were caught, suggesting that the localization of the drug-containing particles result in higher drug concentrations in the cells possibly for extended times. The alpha-TCP particles system is expected to be a good candidate for targeting chemotherapy and specially for abdominal carcinomatosis.     

A 10 b 50 MHz pipelined CMOS A/D converter with S/H

A single 5 V, 10 b, 50 MHz pipelined CMOS analog-to-digital (A/D) converter with internal sample-and-hold (S/H) circuits was developed. The A/D converter features a newly developed S/H circuit with an 80 dB, 300 MHz operational amplifier, three-stage pipelined 4 b flash A/D converters with digital error correction functions, and double analog signal conversion paths whose operations are interleaved. The new A/D converter was fabricated with 0.8 μm CMOS technology     

A capillary electrophoretic reactor with an electroosmosis control method for measurement of dissociation kinetics of metal complexes

The solvolytic dissociation rate constants of 1:2 complexes of Al3+ and Ga3+ with an azo dye ligand, 2,2'-dihydroxyazobenzene-5,5'-disulfonate (DHABS, H2L2-), have been evaluated with a capillary electrophoretic reactor (CER) system. This CER system is based on the fact that metal complexes encounter an overwhelming force to dissociate when apart from the ligand by CE resolution. Treatment of a capillary with a slightly acidic buffer solution, e.g., pH 5, reduces the double-layer potential (zeta) of the inner silica wall. Owing to slow relaxation of the deprotonation equilibria of superficial silanol groups known as the pH hysteresis, this zeta potential can be actually retained during the electrophoresis of the metal complexes in question with a neutral buffer at pH 7.0. This method enables one to manipulate migration times, namely, residence times in a capillary tube, from 5 to 90 min, depending on the prescribed conditioning pH, without changing any other operation conditions such as buffer composition and electric field strength. The excellent performance of the CER is exemplified by the accurate estimation of the dissociation degree of the complexes. The dissociation degree-time profiles for the complexes are quantitatively described using both internal and external standards; the very inert complex of [Co(III)L2]5- for the peak signal standardization and methyl orange for the injection volume correction. The solvolytic dissociation rate constants of the 1:2 complexes of Al3+ and Ga3+ ions with DHABS [AlL2]5- and [GaL2]5- into the 1:1 ones have been determined as (4.9+/-1.0) x 10(-4) and (3.7+/-0.3) x 10(-3) s(-1) at 303 K, respectively.     

Cationic liposomes in gene delivery

Cationic liposomes have been extensively explored as gene delivery vector for several reasons. It is because disadvantages of viral vectors include risk of replication, possible immunogenicity, and the difficulty of obtaining a large quantity of viral vectors. Currently, a variety of cationic components for liposome formulations have been developed. The components are broadly divided into two classes based on the chemical structure of hydrophobic moieties: long aliphatic (saturated or unsaturated) hydrocarbons and cholesterol ring. A variety of hydrophilic moieties also include tertiary amines, ammonium salt and spermine. The role of liposomes is to condense DNA to form complexes with high affinity to cell surfaces where possible fusion or destabilization of the membrane and/or endocytosis are involved. However, at present, little structure-activity relationships are known. Some vectors are on clinical trials approved by NIH.