Your search keyword '"HPLC, high-performance liquid chromatography"' showing total 335 results

101. Advanced oxidation processes for sample treatment in atomic spectrometry

Author

Capelo-Martínez, J.L., Ximénez-Embún, P., Madrid, Y., and Cámara, C.

Subjects

*OXIDATION, *ANALYTICAL chemistry, *PHYSICAL sciences, *OXIDIZING agents

Abstract

Advanced oxidation processes (AOPs), which involve the in situ generation of highly potent chemical oxidants, such as the hydroxyl radical (⋅OH), have emerged as an important class of sample treatments in atomic spectrometry. This article introduces the state-of-the-art of the main AOPs used in analytical chemistry along with an in-depth review of the most representative works published for each of the AOPs selected and some guidelines regarding their near-term future. [Copyright &y& Elsevier]

Published

2004

102. Conformational mapping of the N-terminal peptide of HIV-1 gp41 in lipid detergent and aqueous environments using 13C-enhanced Fourier transform infrared spectroscopy.

Author

Gordon, Larry M., Mobley, Patrick W., Lee, William, Eskandari, Sepehr, Kaznessis, Yiannis N., Sherman, Mark A., and Waring, Alan J.

Abstract

The N-terminal domain of HIV-1 glycoprotein 41,000 (gp41) participates in viral fusion processes. Here, we use physical and computational methodologies to examine the secondary structure of a peptide based on the N terminus (FP; residues 1-23) in aqueous and detergent environments. 12C-Fourier transform infrared (FTIR) spectroscopy indicated greater α-helix for FP in lipid-detergent sodium dodecyl sulfate (SDS) and aqueous phosphate-buffered saline (PBS) than in only PBS. 12C-FTIR spectra also showed disordered FP conformations in these two environments, along with substantial β-structure for FP alone in PBS. In experiments that map conformations to specific residues, isotope-enhanced FTIR spectroscopy was performed using FP peptides labeled with 13C-carbonyl. 13C-FTIR results on FP in SDS at low peptide loading indicated α-helix (residues 5 to 16) and disordered conformations (residues 1-4). Because earlier 13C-FTIR analysis of FP in lipid bilayers demonstrated α-helix for residues 1-16 at low peptide loading, the FP structure in SDS micelles only approximates that found for FP with membranes. Molecular dynamics simulations of FP in an explicit SDS micelle indicate that the fraying of the first three to four residues may be due to the FP helix moving to one end of the micelle. In PBS alone, however, electron microscopy of FP showed large fibrils, while 13C-FTIR spectra demonstrated antiparallel β-sheet for FP (residues 1-12), analogous to that reported for amyloid peptides. Because FP and amyloid peptides each exhibit plaque formation, α-helix to β-sheet interconversion, and membrane fusion activity, amyloid and N-terminal gp41 peptides may belong to the same superfamily of proteins. [ABSTRACT FROM AUTHOR]

Published

2004

103. vAL-1, a novel polysaccharide lyase encoded by chlorovirus CVK2

Author

Sugimoto, Ichiro, Onimatsu, Hideki, Fujie, Makoto, Usami, Shoji, and Yamada, Takashi

Subjects

*POLYSACCHARIDES, *ENZYMES, *CHLORELLA, *SPECTROMETRY

Abstract

Cell wall materials isolated from Chlorella cells were degraded by the polysaccharide-degrading enzyme vAL-1 encoded by chlorovirus CVK2. Matrix-assisted laser desorption/ionization time-of-flight mass spectrometric analyses of the degradation products (oligosaccharides) revealed major oligosaccharides contain unsaturated GlcA at the reducing terminus, and a side chain attached at C2 or C3 of GlcA(C4&z.dbnd6;C5), which mainly consisted of Ara, GlcNAc and Gal. The results indicated that vAL-1 is a novel polysaccharide lyase, cleaving chains of β- or α-1,4-linked GlcAs. The unique structures of Chlorella cell wall were also revealed. Studies on the complicated structures of naturally occurring polysaccharides will be greatly facilitated by using vAL-1 as a tool in structural analysis. [Copyright &y& Elsevier]

Published

2004

104. Lipid raft-associated catechin suppresses the Fc∊RI expression by inhibiting phosphorylation of the extracellular signal-regulated kinase1/2

Author

Fujimura, Yoshinori, Tachibana, Hirofumi, and Yamada, Koji

Subjects

*CATECHIN, *PLASMONS (Physics), *GENE expression, *ALLERGIES

Abstract

The major green tea catechin, (−)-epigallocatechin-3-O-gallate (EGCG), has a suppressive effect on the expression of the high-affinity IgE receptor Fc∊RI, which is key molecule in the IgE-mediated allergic reactions. Here we show that EGCG binds to the cell surface and highly associates with plasma membrane microdomains, lipid rafts, on the human basophilic KU812 cells. The disruption of these lipid rafts caused a reduction of the amount of raft-associated EGCG and the Fc∊RI-suppressive effect of EGCG. We also found that EGCG has an ability to inhibit the phosphorylation of the extracellular signal-regulated kinase1/2 (ERK1/2) and that the ERK1/2 specific inhibitor also reduced Fc∊RI expression. Moreover, the inhibitory effect elicited by EGCG on ERK1/2 was prevented by disruption of rafts. Thus, these results suggest that the interaction between EGCG and the lipid rafts is important for EGCG’s ability to downregulate Fc∊RI expression, and ERK1/2 may be involved in this suppression signal. [Copyright &y& Elsevier]

Published

2004

105. Design, synthesis, and biological evaluation of quinazolin-4(3

Author

Xiaosa, Chang, Dejuan, Sun, Danfeng, Shi, Guan, Wang, Yanmei, Chen, Kai, Zhang, Huidan, Tan, Jie, Liu, Bo, Liu, and Liang, Ouyang

Subjects

Synthetic lethality, DSB, DNA double-strand break, ER, estrogen receptor, HRD, homologous recombination deficiency, BC, breast cancer, Dual-target inhibitor, PARP1, TNBC, triple-negative breast cancer, PI, propidium iodide, HE, hematoxylin-eosin, Quinazolin-4(3H)-one derivatives, CDK4/6, cyclin-dependent kinase 4/6, SAR, structure–activity relationship, ELISA, enzyme linked immunosorbent assay, BRD4, bromodomain 4, TCGA, the cancer genome atlas, TGI, tumor growth inhibition, TR-FRET, time-resolved fluorescence resonance energy transfer, FITC, fluorescein isothiocyanate isomer I, BET, bromodomain and extra-terminal domain, TLC, thin-layer chromatography, PPI, protein−protein interaction, ESI-HR-MS, high-resolution mass spectra, EGFR, epidermal growth factor receptor, FDA, U.S. Food and Drug Administration, SOP, standard operation process, HPLC, high-performance liquid chromatography, shRNA, short hairpin RNA, BRD4, PK, pharmacokinetics, Original Article, BRCA1/2, breast cancer susceptibility gene 1/2, NHEJ, nonhomologous end-joining, HR, homologous recombination, PARP1, poly(ADP-ribose) polymerase-1, IHC, immunohistochemistry

Abstract

This study was aimed to design the first dual-target small-molecule inhibitor co-targeting poly (ADP-ribose) polymerase-1 (PARP1) and bromodomain containing protein 4 (BRD4), which had important cross relation in the global network of breast cancer, reflecting the synthetic lethal effect. A series of new BRD4 and PARP1 dual-target inhibitors were discovered and synthesized by fragment-based combinatorial screening and activity assays that together led to the chemical optimization. Among these compounds, 19d was selected and exhibited micromole enzymatic potencies against BRD4 and PARP1, respectively. Compound 19d was further shown to efficiently modulate the expression of BRD4 and PARP1. Subsequently, compound 19d was found to induce breast cancer cell apoptosis and stimulate cell cycle arrest at G1 phase. Following pharmacokinetic studies, compound 19d showed its antitumor activity in breast cancer susceptibility gene 1/2 (BRCA1/2) wild-type MDA-MB-468 and MCF-7 xenograft models without apparent toxicity and loss of body weight. These results together demonstrated that a highly potent dual-targeted inhibitor was successfully synthesized and indicated that co-targeting of BRD4 and PARP1 based on the concept of synthetic lethality would be a promising therapeutic strategy for breast cancer., Graphical abstract The first potential BRD4 and PARP1 inhibitors 19d named ADTL-BPI1901 was discovered and synthesized by fragment-based combinatorial screening and activity assays led to the three rounds of structural optimization. Preliminary structure−activity relationships, molecular modeling, pharmacokinetics and favorable in vivo antitumor efficacy of 19d were investigated.Image 1

Published

2020

106. Remote loading paclitaxel-doxorubicin prodrug into liposomes for cancer combination therapy

Author

Guimei Lin, Xue Wang, Zhonggui He, Yongjun Wang, Dongxu Chi, Shuang Zhou, Yingli Wang, Jinbo Li, Jiamei Wang, and Jiang Yu

Subjects

BUN, blood urea nitrogen, DL, drug loading, IC50, half maximal inhibitory concentration, CO2, carbon dioxide, DMSO, dimethyl sulfoxide, Pharmacology, AUC, area under the curve, DTT, d,l-dithiothreitol, EDTA, ethylene diamine tetraacetic acid, MTT, 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide, chemistry.chemical_compound, DNA, deoxyribonucleic acid, 0302 clinical medicine, Remote loading liposomes, AST, aspartate transaminase, GSH, glutathione, General Pharmacology, Toxicology and Pharmaceutics, Prodrug, HSPC, hydrogenated soybean phospholipids, DLS, dynamic light scattering, 0303 health sciences, Liposome, DSPE-PEG2000, 2-distearoyl-snglycero-3-phosphoethanolamine-N-[methyl(polyethylene glycol)-2000, musculoskeletal, neural, and ocular physiology, MTD, maximum tolerated dose, Combination chemotherapy, PSD, PTX-S-DOX, PSD LPs, PTX-S-DOX liposomes, Paclitaxel, H2O2, hydrogen peroxide, 030220 oncology & carcinogenesis, Original Article, MRT, mean residence time, Safety, psychological phenomena and processes, medicine.drug, Combination therapy, ALT, alanine transaminase, CR, creatinine, IVIS, in vivo imaging system, Paclitaxel–doxorubicin prodrug, 03 medical and health sciences, PBS, phosphate buffer saline, ROS, reactive oxygen species, FBS, fetal bovine serum, Pharmacokinetics, mental disorders, medicine, Doxorubicin, MLVs, multilamellar vesicles, TEM, transmission electron microscopy, 030304 developmental biology, Cardiotoxicity, CHO, cholesterol, PSD NPs, PTX-S-DOX self-assembled nanoparticles, lcsh:RM1-950, HEPES, 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid, PDI, polydispersity index, DOX, doxorubicin, UV, ultraviolet, PTX, paclitaxel, lcsh:Therapeutics. Pharmacology, EE, encapsulation efficacy, chemistry, nervous system, HPLC, high-performance liquid chromatography, H&E, hematoxylin and eosin, Nanoparticles, Cu2+, copper ions, SD, standard deviation

Abstract

The combination of paclitaxel (PTX) and doxorubicin (DOX) has been widely used in the clinic. However, it remains unsatisfied due to the generation of severe toxicity. Previously, we have successfully synthesized a prodrug PTX-S-DOX (PSD). The prodrug displayed comparable in vitro cytotoxicity compared with the mixture of free PTX and DOX. Thus, we speculated that it could be promising to improve the anti-cancer effect and reduce adverse effects by improving the pharmacokinetics behavior of PSD and enhancing tumor accumulation. Due to the fact that copper ions (Cu2+) could coordinate with the anthracene nucleus of DOX, we speculate that the prodrug PSD could be actively loaded into liposomes by Cu2+ gradient. Hence, we designed a remote loading liposomal formulation of PSD (PSD LPs) for combination chemotherapy. The prepared PSD LPs displayed extended blood circulation, improved tumor accumulation, and more significant anti-tumor efficacy compared with PSD NPs. Furthermore, PSD LPs exhibited reduced cardiotoxicity and kidney damage compared with the physical mixture of Taxol and Doxil, indicating better safety. Therefore, this novel nano-platform provides a strategy to deliver doxorubicin with other poorly soluble antineoplastic drugs for combination therapy with high efficacy and low toxicity., Graphical abstract The authors designed a remote loading paclitaxel–doxorubicin prodrug liposomal formulation for combination of PTX and DOX. The prodrug could respond to high ROS/GSH of the tumor microenvironment. The stimuli-responsive liposomes were proved to be a high-efficacy and low-toxicity formulation. This technology provides a novel pathway for cancer combination therapy.Image 1

Published

2020

107. Peptide models of four possible insulin folding intermediates with two disulfides.

Author

Jia, Xiao-Yuan, Guo, Zhan-Yun, Wang, Yao, Xu, Ye, Duan, Shun-Shan, and Feng, You-Min

Abstract

The single-chain insulin (PIP) can spontaneously fold into native structure through preferred kinetic intermediates. During refolding, pairing of the first disulfide A20-B19 is highly specific, whereas pairing of the second disulfide is likely random because two two-disulfide intermediates have been trapped. To get more details of pairing property of the second disulfide, four model peptides of possible folding intermediates with two disulfides were prepared by protein engineering, and their properties were analyzed. The four model peptides were named [A20-B19, A7-B7]PIP, [A20-B19, A6-B7]PIP, [A20-B19, A6-A11]PIP, and [A20-B19, A7-A11]PIP according to their remaining disulfides. The four model peptides all adopt partially folded structure with moderate conformational differences. In redox buffer, the disulfides of the model peptides are more easily reduced than those of the wild-type PIP. During in vitro refolding, the reduced model peptides share similar relative folding rates but different folding yields: The refolding efficiency of the reduced [A20-B19, A7-A11]PIP is about threefold lower than that of the other three peptides. The present results indicate that the folding intermediates corresponding to the present model peptides all adopt partially folded conformation, and can be formed during PIP refolding, but the chance of forming the intermediate with disulfide [A20-B19, A7-A11] is much lower than that of forming the other three intermediates. [ABSTRACT FROM AUTHOR]

Published

2003

108. Separation of the yellow chromophores in individual brunescent cataracts

Author

Cheng, Rongzhu, Lin, Bin, and Ortwerth, Beryl J.

Subjects

*CATARACT, *PROTEINS, *EYE

Abstract

Quantitative changes in the 330 nm absorbing chromophores and 350/450 nm fluorophores of water-soluble (WS) and water-insoluble (WI) proteins of individual human cataract lenses were characterized and compared with aged normal human lens. Twenty-five brunescent cataract lenses from India were selected from five different stages (types I–V) based upon the color of the lens. The WS and WI proteins from each lens were collected and subjected to an extensive enzymatic digestion procedure under argon. The lens protein digests were separated by Bio-Gel P-2 size-exclusion chromatography and individual peaks were analyzed further by reversed-phase HPLC. The total WI proteins increased and the total WS protein decreased with the development of cataract, especially in the late stages of cataract (III–V). The total 330 nm absorbance and 350/450 nm fluorescence of the WI fraction also increased, however, the A330 and fluorescence per mg lens protein were constant except for type V (black) lenses. Bio-Gel P-2 chromatography separated the chromophores and fluorophores into four fractions. The main fraction (designated as peak 2+3) from the cataract WI proteins was several times higher than that present in aged normal human lens WI proteins. A significant increase of this fraction was observed in WI proteins, but not in WS proteins with cataract development. Similarly, fractions 1 and 4 in the WI proteins also increased gradually but fraction 5 did not. Reversed-phase HPLC resolved fraction (2+3) of the water-insoluble sonicate supernatant proteins into four 330 nm absorbing peaks and eight fluorescent peaks. Among these peaks, a late-eluting peak (peak 8) increased 10 to 15-fold with the progress of cataract, and accounted for 80% of the total chromophores in type V lenses. This peak may represent limit digests of advanced glycation end-products (AGEs) derived protein cross-links. HPLC profiles of fraction 5 from both WS and WI proteins showed numerous new peaks which were not observed in either WS protein from cataract or WI proteins from aged normal human. The severe coloration and the higher levels of numerous novel chromophores and fluorophores in brunescent cataractous lenses reveal the possibility that a different chemistry occurs during cataract development. [Copyright &y& Elsevier]

Published

2003

109. Solution structure of Pi4, a short four-disulfide-bridged scorpion toxin specific of potassium channels.

Author

Guijarro, J. Iñaki, M'Barek, Sarrah, Gómez-Lagunas, Froylan, Garnier, Damien, Rochat, Hervé, Sabatier, Jean-Marc, Possani, Lourrival D., and Delepierre, Muriel

Abstract

Pi4 is a short toxin found at very low abundance in the venom of Pandinus imperator scorpions. It is a potent blocker of K+ channels. Like the other members of the α-KTX6 subfamily to which it belongs, it is cross-linked by four disulfide bonds. The synthetic analog (sPi4) and the natural toxin (nPi4) have been obtained by solid-phase synthesis or from scorpion venom, respectively. Analysis of two-dimensional 1H NMR spectra of nPi4 and sPi4 indicates that both peptides have the same structure. Moreover, electrophysiological recordings of the blocking of Shaker B K+ channels by sPi4 (KD = 8.5 nM) indicate that sPi4 has the same blocking activity of nPi4 (KD = 8.0 nM), previously described. The disulfide bonds have been independently determined by NMR and structure calculations, and by Edman-degradation/mass-spectrometry identification of peptides obtained by proteolysis of nPi4. Both approaches indicate that the pairing of the half-cystines is 6C-27C, 12C-32C, 16C-34C, and 22C-37C. The structure of the toxin has been determined by using 705 constraints derived from NMR data on sPi4. The structure, which is well defined, shows the characteristic α/β scaffold of scorpion toxins. It is compared to the structure of the other α-KTX6 subfamily members and, in particular, to the structure of maurotoxin, which shows a different pattern of disulfide bridges despite its high degree of sequence identity (76%) with Pi4. The structure of Pi4 and the high amounts of synthetic peptide available, will enable the detailed analysis of the interaction of Pi4 with K+ channels. [ABSTRACT FROM AUTHOR]

Published

2003

110. Identification of S-sulfonation and S-thiolation of a novel transthyretin Phe33Cys variant from a patient diagnosed with familial transthyretin amyloidosis.

Author

Lim, Amareth, Prokaeva, Tatiana, McComb, Mark E., Connors, Lawreen H., Skinner, Martha, and Costello, Catherine E.

Abstract

Familial transthyretin amyloidosis (ATTR) is an autosomal dominant disorder associated with a variant form of the plasma carrier protein transthyretin (TTR). Amyloid fibrils consisting of variant TTR, wild-type TTR, and TTR fragments deposit in tissues and organs. The diagnosis of ATTR relies on the identification of pathologic TTR variants in plasma of symptomatic individuals who have biopsy proven amyloid disease. Previously, we have developed a mass spectrometry-based approach, in combination with direct DNA sequence analysis, to fully identify TTR variants. Our methodology uses immunoprecipitation to isolate TTR from serum, and electrospray ionization and matrix-assisted laser desorption/ionization mass spectrometry (MS) peptide mapping to identify TTR variants and posttranslational modifications. Unambiguous identification of the amino acid substitution is performed using tandem MS (MS/MS) analysis and confirmed by direct DNA sequence analysis. The MS and MS/MS analyses also yield information about posttranslational modifications. Using this approach, we have recently identified a novel pathologic TTR variant. This variant has an amino acid substitution (Phe → Cys) at position 33. In addition, like the Cys10 present in the wild type and in this variant, the Cys33 residue was both S-sulfonated and S-thiolated (conjugated to cysteine, cysteinylglycine, and glutathione). These adducts may play a role in the TTR fibrillogenesis. [ABSTRACT FROM AUTHOR]

Published

2003

111. [35S]-Labeling of the Salmonella typhimurium glutathione pool to assess glutathione-mediated DNA binding by 1,2-dibromoethane

Author

Ross, Matthew K. and Pegram, Rex A.

Subjects

*BIOTRANSFORMATION (Metabolism), *CHEMICALS, *GLUTATHIONE

Abstract

Biotransformation of drugs and environmental chemicals to reactive intermediates is often studied with the use of radiolabeled compounds that are synthesized by expensive and technically difficult procedures. In general, glutathione (GSH) conjugation serves as a detoxification mechanism, and conjugation of reactive intermediates with GSH is often a surrogate marker of reactive species formation. However, several halogenated alkanes can be bioactivated by GSH to yield highly reactive GSH conjugates, some of which are DNA-reactive (e.g. conjugates of 1,2-dibromoethane). The purpose of this study was to metabolically radiolabel the in vivo GSH pool of Salmonella typhimurium with a [35S]-label and to examine the GSH-mediated bioactivation of a model haloalkane, 1,2-dibromoethane, by measuring the binding of [35S]-label to DNA. The strain of Salmonella used in this study had been transformed previously with the gene that codes for rat glutathione transferase theta 1-1 (GSTT1-1), an enzyme that can catalyze formation of genotoxic GSH conjugates. Bacteria were grown to mid-log phase and then incubated with [35S]-l-cysteine in minimal medium (thio-free) until stationary phase of growth was reached. At this stage, the specific activity of Salmonella GSH was estimated to be 7.1 mCi/mmol by derivatization and subsequent HPLC analysis, and GSTT1-1 enzyme activity was still demonstrable in Salmonella cytosol following growth in a minimal medium. The [35S]-labeled bacteria were then exposed to 1,2-dibromoethane (1 mM), and the Salmonella DNA was subsequently purified to quantify [35S]-binding to DNA. The amount of [35S]-label that was covalently bound to DNA in the GSTT1-1-expressing Salmonella strain (33.2 nmol/mg DNA) was sevenfold greater than that of the control strain that does not express GSTT1-1. Neutral thermal hydrolysis of the DNA yielded a single [35S]-labeled adduct with a similar tR as S-[2-(N7-guanyl)ethyl]GSH, following HPLC analysis of the hydrolysate. This adduct accounted for 95% of the total [35S]-label bound to DNA. Thus, this [35S]-radiolabeling protocol may prove useful for studying the DNA reactivity of GSH conjugates of other halogenated alkanes in a cellular context that maintains GSH at normal physiological levels. This is also, to our knowledge, the first demonstration of de novo incorporation of [35S]-l-cysteine into the bacterial GSH pool. [Copyright &y& Elsevier]

Published

2003

112. Detection of DNA methylation changes during somatic embryogenesis of Siberian ginseng (Eleuterococcus senticosus)

Author

Chakrabarty, Debasis, Yu, K.W., and Paek, K.Y.

Subjects

*PLANTS, *GROWTH

Abstract

DNA methylation is known to play an important role in the regulation of gene expression in eukaryotes. In this study, we assessed the extent and pattern of cytosine methylation during somatic embryogenesis in Eleuterococcus senticosus, using two methods to evaluate DNA methylation rates: (1) direct determination of 5-methyl-deoxycytidine (5mdC) amounts in genomic DNA by HPLC separation and quantification of nucleosides and (2) methylation-sensitive amplification polymorphism (MSAP) technique. The tissue assayed include embryogenic and non-embryogenic callus. Leaf segments were cultured on modified Murashige and Skoog (MS) medium containing 2,4-dichlorophenoxyacetic acid (2,4-D). Opaque and friable embryogenic callus formed on modified MS medium with 2.26 μM 2,4-D. Initiation and development of somatic embryos occurred in the same medium containing 2.26 μM 2,4-D. Non-embryogenic callus failed to regenerate even after prolonged maintenance and subculture on to the same media. Dark treatment significantly increased the number of mature somatic embryos. HPLC analyses on genomic DNA from embryogenic and non-embryogenic callus showed that global DNA methylation rates were significantly lowered in embryogenic calli. Similarly, 16.99% of 5′-CCGG-3 sites in the genome of non-embryogenic callus were cytosine methylated, where as 11.20% were methylated in case of embryogenic callus tissue, as detected by MSAP technique. Hypermethylation of DNA in non-embryogenic callus compared with embryogenic callus reflects the marked expression of this molecular feature, which may well contribute to the developmental gene expression. [Copyright &y& Elsevier]

Published

2003

113. Unique stabilizing interactions identified in the two-stranded α-helical coiled-coil: Crystal structure of a cortexillin I/GCN4 hybrid coiled-coil peptide.

Author

Lee, Darin L., Ivaninskii, Sergei, Burkhard, Peter, and Hodges, Robert S.

Abstract

We determined the 1.17 Å resolution X-ray crystal structure of a hybrid peptide based on sequences from coiled-coil regions of the proteins GCN4 and cortexillin I. The peptide forms a parallel homodimeric coiled-coil, with Cα backbone geometry similar to GCN4 (rmsd value 0.71 Å). Three stabilizing interactions have been identified: a unique hydrogen bonding-electrostatic network not previously observed in coiled-coils, and two other hydrophobic interactions involving leucine residues at positions e and g from both g-a' and d-e' interchain interactions with the hydrophobic core. This is also the first report of the quantitative significance of these interactions. The GCN4/cortexillin hybrid surprisingly has two interchain Glu-Lys' ion pairs that form a hydrogen bonding network with the Asn residues in the core. This network, which was not observed for the reversed Lys-Glu' pair in GCN4, increases the combined stability contribution of each Glu-Lys' salt bridge across the central Asn15-Asn15′ core to ∼0.7 kcal/mole, compared to ∼0.4 kcal mole−1 from a Glu-Lys' salt bridge on its own. In addition to electrostatic and hydrogen bonding stabilization of the coiled-coil, individual leucine residues at positions e and g in the hybrid peptide also contribute to stability by 0.7 kcal/mole relative to alanine. These interactions are of critical importance to understanding the stability requirements for coiled-coil folding and in modulating the stability of de novo designed macromolecules containing this motif. [ABSTRACT FROM AUTHOR]

Published

2003

114. Subsite mapping of human salivary α-amylase and the mutant Y151M

Author

Kandra, Lili, Gyémánt, Gyöngyi, Remenyik, Judit, Ragunath, Chandran, and Ramasubbu, Narayanan

Subjects

*SALIVARY glands, *FORCE & energy

Abstract

This study characterizes the substrate-binding sites of human salivary α-amylase (HSA) and its Y151M mutant. It describes the first subsite maps, namely, the number of subsites, the position of cleavage sites and apparent subsite energies. The product pattern and cleavage frequencies were determined by high-performance liquid chromatography, utilizing a homologous series of chromophore-substituted maltooligosaccharides of degree of polymerization 3–10 as model substrates. The binding region of HSA is composed of four glycone and three aglycone-binding sites, while that of Tyr151Met is composed of four glycone and two aglycone-binding sites. The subsite maps show that Y151M has strikingly decreased binding energy at subsite (+2), where the mutation has occurred (−2.6 kJ/mol), compared to the binding energy at subsite (+2) of HSA (−12.0 kJ/mol). [Copyright &y& Elsevier]

Published

2003

115. Inhibition of oxidized LDL aggregation with the calcium channel blocker amlodipine: role of electrostatic interactions

Author

Phillips, Jane Ellen and Preston Mason, R.

Subjects

*LIPOPROTEINS, *CHOLESTEROL

Abstract

Atherogenic low-density lipoproteins (LDL) are characterized by elevations in cholesterol content and increased electronegativity, factors that contribute to aggregation and foam cell formation. This study was designed to test the effect of the positively charged calcium channel blocker (CCB) amlodipine on the aggregation properties of oxidized LDL lipids. Large unilamellar vesicles (LUVs) (100 nm diameter) labeled with a non-exchangeable marker [3H]cholesteryl hexadecyl ether were prepared with lipids extracted from human LDL following oxidation. The LUVs were shown to bind, in a reversible fashion, to charged diethylaminoethyl Sephadex columns. The addition of amlodipine inhibited binding of the oxidized LDL lipids in a dose-dependent fashion with an IC50 in the nanomolar range as a result of its high lipophilicity and positively charged amino group (pKa of 9.02). The activity of amlodipine was reproduced in model membranes that contained fixed amounts of charged phospholipid (glycerophospholipid) in a concentration-dependent manner. By contrast, drugs lacking a formal positive charge, including CCBs (felodipine, nifedipine, diltiazem, verapamil) and an angiotensin-converting enzyme-inhibitor (ramiprilate) had no effect on the column binding of the modified, electronegative lipids. These effects of amlodipine on LDL lipid aggregation and electrostatic properties may represent a novel antiatherosclerotic mechanism of action. [Copyright &y& Elsevier]

Published

2003

116. Complementation of Escherichia coli ubiF mutation by Caenorhabditis elegans CLK-1, a product of the longevity gene of the nematode worm

Author

Adachi, Akihiko, Shinjyo, Noriko, Fujita, Daisuke, Miyoshi, Hideto, Amino, Hisako, Watanabe, Yoh-ichi, and Kita, Kiyoshi

Subjects

*BIOSYNTHESIS, *PROTEINS

Abstract

Caenorhabditis elegans CLK-1 was identified from long-lived mutant worms, and is believed to be involved in ubiquinone biosynthesis. The protein belongs to the eukaryotic CLK-1/Coq7p family, which is also similar to the bacterial Coq7 family, that hydroxylates demethoxyubiquinone, resulting in the formation of hydroxyubiquinone, a precursor of ubiquinone. In Escherichia coli, the corresponding reaction is catalyzed by UbiF, a member of a distinct class of hydroxylase. Although previous studies suggested that the eukaryotic CLK-1/Coq7 family is a hydroxylase of demethoxyubiquinone, there was no direct evidence to show the enzymatic activity of the eukaryotic CLK-1/Coq7 family. Here we show that the plasmid encoding C. elegans CLK-1 supported aerobic respiration on a non-fermentable carbon source of E. coli ubiF mutant strain and rescued the ability to synthesize ubiquinone, suggesting that the eukaryotic CLK-1/Coq7p family could function as bacterial UbiF. [Copyright &y& Elsevier]

Published

2003

117. Efficacy of a glycyrrhizin suppository for the treatment of chronic hepatitis C: a pilot study

Author

Fujioka, Takahiro, Kondou, Toshirou, Fukuhara, Akinori, Tounou, Shigetaka, Mine, Masafumi, Mataki, Norikazu, Hanada, Kenji, Ozaka, Masato, Mitani, Keiji, Nakaya, Teruo, Iwai, Tomohisa, and Miyakawa, Hiroshi

Subjects

*INTRAVENOUS therapy, *SERUM, *AMINOTRANSFERASES, *HEPATITIS, *SALT

Abstract

Intravenous administration of glycyrrhizin has potential efficacy on decreasing serum aminotransferase levels in patients with chronic hepatitis. However, patients receiving this treatment are recommended to attend hospital regularly for several years. To improve the quality of life for these patients, we developed a glycyrrhizin suppository. In this pilot study, we examined the most effective and safe material contents of the suppository and revealed clinical efficacy for patients with biopsy-proven chronic hepatitis C comparing intravenous administration of glycyrrhizin. As content combinations of the suppository, a mixture of 300 mg of glycyrrhizinic ammonium salt and 60 μg of sodium capric acid, with pH neutralization, was confirmed to be most effective and safe condition, based on analysis of serum glycyrrhizin levels and the grade of rectal irritations in tested patients. The efficacy on decreasing serum alanine aminotransferase levels for 12-week administration of the suppository in 13 patients with chronic hepatitis C was similar to that in another 13 patients intravenously administered glycyrrhizin. Moreover, no serious side effects were observed. In conclusion, the usage of the newly developed suppository of glycyrrhizin can improve the quality of life for chronic hepatitis C patients, especially those who do not respond with viral clearance to interferon therapy. Using this suppository, larger and longer-term studies are needed. [Copyright &y& Elsevier]

Published

2003

118. Liposome entrapment and immunogenic studies of a synthetic lipophilic multiple antigenic peptide bearing VP1 and VP3 domains of the hepatitis A virus: a robust method for vaccine design

Author

Haro, Isabel, Pérez, Silvia, García, Mónica, Chan, Weng C., and Ercilla, Guadalupe

Subjects

*HEPATITIS A virus, *PEPTIDES

Abstract

Multiple antigen peptides (MAP) have been demonstrated to be efficient immunological reagents for the induction of immune responses to a variety of infectious agents. Several peptide domains of the hepatitis A virus (HAV) capsid proteins, mainly VP1 and VP3, are the immunodominant targets for a protective antibody response. In the present study we analyse the immunogenic properties of a tetrameric heterogeneous palmitoyl-derivatised MAP containing two defined HAV peptide sequences, VP1(11–25) and VP3(102–121), in rabbits immunised with either Freund’s adjuvant or multilamellar liposomes. The immune response was evaluated with a specific enzyme immunoassay using MAP[VP1+VP3], VP1 and VP3 as targets. The avidity of the immune response was measured by a non-competitive enzyme-linked immunosorbent assay and by the surface plasmon resonance technology. Antisera raised against the lipo-MAP peptide entrapped in liposomes demonstrated high avidity of binding with affinity rate constants approximately one order of magnitude greater than those obtained with the Freund’s protocol. [Copyright &y& Elsevier]

Published

2003

119. Matrix deposition of tryptophan-containing allelic variants of type IX collagen in developing human cartilage

Author

Matsui, Yoshito, Wu, Jiann-Jiu, Ann Weis, Mary, Pietka, Terri, and Eyre, David R.

Subjects

*GENETIC polymorphisms, *EXTRACELLULAR matrix

Abstract

Genetic polymorphisms that encode a tryptophan (Trp) residue in the triple-helical domain of the α2 (Trp2) or α3 chain (Trp3) of human type IX collagen have been linked to risk of degenerative intervertebral disc disease. To determine whether these two allelic variants express protein that may affect the extracellular matrix of cartilage in vivo, we examined the properties of resident type IX collagen in an anonymous collection of embryonic and fetal human cartilage samples screened for Trp genotypes. No difference was found in the yield and electrophoretic properties of pepsin-solubilized type IX collagen between Trp2, Trp3 and non-Trp cartilage samples. On Western blot analysis, a polyclonal antiserum raised against a synthetic peptide matching the immediate Trp-containing sequence of the Trp3 allele reacted specifically with the α3(IX) chain prepared from Trp3 cartilage samples. Two-dimensional peptide mapping of type IX collagen in CNBr-digests of whole tissue gave indistinguishable fingerprints for Trp2, Trp3 and control tissues, including the yield of cross-linked peptides. Analysis of one cartilage sample that was homozygous for the Trp2 allele also gave a normal yield of collagen IX, including its α2 chain and a normal profile of cross-linked peptides. Together, the findings indicate that both Trp2 and Trp3 allelic products are incorporated into the cross-linked fibrillar network of developing human cartilage apparently normally. Any pathological consequences are likely, therefore, to be long-term and indirect rather than from overt misassembly of matrix. [Copyright &y& Elsevier]

Published

2003

120. Improved method for measurement of human plasma xanthine oxidoreductase activity

Author

Liu, X., Lin, W.M., Yan, X.H., Chen, X.H., Hoidal, J.R., and Xu, P.

Subjects

*URIC acid, *BLOOD plasma, *OXIDOREDUCTASES, *XANTHINE

Abstract

The XOR activity in human plasma was measured by quantifying the XOR-derived uric acid (UA) in plasma using the high-performance liquid chromatography (HPLC) equipped with a UV detector. Chromatographic separation consisted of the mobile phase (a mixture of 0.1% trifluoroacetic acid in Milli-Q water and 0.085% trifluoroacetic acid in acetonitrile in a mix ratio of 99:1) running through a Zorbax StableBond SB-C18 column at a flow-rate of 1 ml/min. Deproteinization with heat-treatment of plasma samples after the reaction was used in the assay to avoid splitting of the UA and xanthine peaks caused by acid deproteinization that could interfere the accurate determination of human plasma XOR activity in our case. Based on the examination of the dependence of XOR activity on added amounts of xanthine and reaction times, the amount of xanthine and reaction time for XOR activity assay were determined to prevent the errors caused by the limiting effect of substrates and plateau phase of the reaction. Using this method, human plasma XOR activities of 25 healthy people were measured. The average human plasma XOR activity was 2.1±0.8 (×10−3 U/ml). [Copyright &y& Elsevier]

Published

2003

121. Stereochemical aspects of carbonyl reduction of the original anticancer drug oracin by mouse liver microsomes and purified 11β-hydroxysteroid dehydrogenase type 1

Author

Wsól, Vladimır, Szotáková, Barbora, Skálová, Lenka, and Maser, Edmund

Subjects

*DEHYDROGENASES, *ELECTROPHORESIS

Abstract

Oracin, 6-[2-(2-hydroxyethyl)aminoethyl]-5,11-dioxo-5,6-dihydro-11H-indeno[1,2-c] isoquinoline, is a potential cytostatic drug for oral use and presently in phase II of clinical trials. Major advantages of this novel chemotherapeutic are the possibility of oral administration, its negative results in the Ames test on mutagenicity, and the lack of cardiotoxicity. Metabolic studies on oracin have revealed that the principal metabolite in all laboratory animals is 11-dihydrooracin (DHO), which is produced by carbonyl reduction of the parent compound. Since the carbonyl moiety of oracin is a pro-chiral centre, reduction may lead to the two stereoisomer forms (+)-DHO and (−)-DHO. The aim of the present study was to infer if 11β-hydroxysteroid dehydrogenase type 1 (11β-HSD 1) is responsible for carbonyl reduction of oracin in mouse liver and if this enzyme exhibits stereospecificity in DHO formation. 11β-HSD 1 was purified from mouse liver microsomes, and the kinetics and stereospecificity regarding DHO formation were determined and compared to values obtained from the whole microsomal fraction. We could show that purified mouse liver 11β-HSD 1 catalyzes the stereospecific carbonyl reduction of oracin, thereby following a sigmoidal dose–response kinetics. Due to a different ratio of (+)-DHO and (−)-DHO (93:7) formed by purified 11β-HSD 1 compared to that produced in whole microsomes (70:30), the existence of at least one other oracin carbonyl reducing enzyme can be expected in mouse liver microsomes. This suggestion is further supported by the fact that the Hill coefficient of 2 for purified 11β-HSD 1 (which is supporting earlier data on the cooperativity of this dimeric enzyme) changes to a Hill coefficient of 3 in whole microsomes (which is indicative for another enzyme participating in oracin carbonyl reduction). [Copyright &y& Elsevier]

Published

2003

122. Differential binding characteristics of protein G and protein A for Fc fragments of papain-digested mouse IgG

Author

Aybay, Cemalettin

Subjects

*PROTEINS, *IMMUNOGLOBULINS

Abstract

It has been previously reported that staphylococcal protein A (SPA) bound only to the Fc region of mouse immunoglobulin G (IgG) and streptococcal protein G (SPG) bound to both Fab and Fc regions of mouse IgG and the binding sites for SPG and SPA on Fc were overlapped. In this study the binding characteristics of SPG and SPA for papain-digested mouse IgG were analysed. Papain digestion of mouse IgG purified from CAy-IFNg99C hybridoma (secreting IgG1 monoclonal antibody specific for human interferon gamma)-induced ascites resulted in Fab and two major Fc fragments referred to as the high molecular weight (HMW) and the low molecular weight (LMW) Fc fragments. SPG bound to Fab and the LMW Fc fragments of the papain-digested IgG. However SPG did not bind to the HMW Fc fragment. SPA showed practically no reactivity with the Fab and the LMW Fc fragments of the papain-digested mouse IgG but only to the HMW Fc fragment. SPG and SPA binding assays showed that papain digestion discriminated the SPG and SPA binding sites in the Fc fragment of mouse IgG. These results demonstrated a clear evidence for the presence of two independent SPG and SPA binding sites in the Fc fragment of mouse IgG. [Copyright &y& Elsevier]

Published

2003

123. Effect of therapeutic drug monitoring on outcome in antiretroviral experienced HIV-infected individuals

Author

Mallon, Patrick W.G., Ray, John, and Cooper, David A.

Subjects

*DRUG monitoring, *RETROVIRUS disease treatment, *THERAPEUTICS, *HIV infections, *REVERSE transcriptase

Abstract

Background: The role of therapeutic drug monitoring (TDM) in the routine management of HIV-infected individuals is still unclear, largely due to a lack of basic data regarding specific drug concentrations and how they correlate with maximal effect and minimal toxicity within given populations. Nevertheless, it has a potentially important role to play in the management of HIV-infected patients, with the aim of limiting toxicity, optimising antiviral effect and decreasing virological failure and emergence of viral resistance. Objectives: To measure serum concentrations of specific antiretroviral drugs in individuals changing antiretroviral therapy and assess relationship to virological response. Study design: A prospective, non-randomised, 24-week study of 40 antiretroviral experienced HIV-infected patients. Subjects had failed their previous antiretroviral regimen and were beginning new regimens based on genotypic testing. Serum antiretroviral concentrations and virological response was measured after initiation of treatment. Results: There was a significant correlation between higher concentrations of lopinavir and efavirenz and better virological outcome. This was not seen with amprenavir. Conclusions: Use of TDM in this setting helps predict virological response to therapy. Optimal use of TDM would require dose adjustment on the basis of a TDM level. Further research is necessary to enable this practice to become routine in the management of HIV-infected patients. [Copyright &y& Elsevier]

Published

2003

124. DsbA and DsbC-catalyzed Oxidative Folding of Proteins with Complex Disulfide Bridge Patterns In Vitro and In Vivo

Author

Maskos, Klaus, Huber-Wunderlich, Martina, and Glockshuber, Rudi

Subjects

*PROTEINS, *ESCHERICHIA coli, *CHEMICAL inhibitors

Abstract

Oxidative protein folding in the periplasm of Escherichia coli is catalyzed by the thiol-disulfide oxidoreductases DsbA and DsbC. We investigated the catalytic efficiency of these enzymes during folding of proteins with a very complex disulfide pattern in vivo and in vitro, using the Ragi bifunctional inhibitor (RBI) as model substrate. RBI is a 13.1 kDa protein with five overlapping disulfide bonds. We show that reduced RBI can be refolded quantitatively in glutathione redox buffers in vitro and spontaneously adopts the single correct conformation out of 750 possible species with five disulfide bonds. Under oxidizing redox conditions, however, RBI folding is hampered by accumulation of a large number of intermediates with non-native disulfide bonds, while a surprisingly low number of intermediates accumulates under optimal or reducing redox conditions. DsbC catalyzes folding of RBI under all redox conditions in vitro, but is particularly efficient in rearranging buried, non-native disulfide bonds formed under oxidizing conditions. In contrast, the influence of DsbA on the refolding reaction is essentially restricted to reducing redox conditions where disulfide formation is rate limiting. The effects of DsbA and DsbC on folding of RBI in E. coli are very similar to those observed in vitro. Whereas overexpression of DsbA has no effect on the amount of correctly folded RBI, co-expression of DsbC enhanced the efficiency of RBI folding in the periplasm of E. coli about 14-fold. Addition of reduced glutathione to the growth medium together with DsbC overexpression further increased the folding yield of RBI in vivo to 26-fold. This shows that DsbC is the bacterial enzyme of choice for improving the periplasmic folding yields of proteins with very complex disulfide bond patterns. [Copyright &y& Elsevier]

Published

2003

125. Whale (Balaenoptera physalus) haemoglobin: primary structure, functional characterisation and computer modelling studies

Author

Corda, Marcella, Tamburrini, Maurizio, De Rosa, Maria C., Sanna, Maria T., Fais, Antonella, Olianas, Alessandra, Pellegrini, Mariagiuseppina, Giardina, Bruno, and di Prisco, Guido

Subjects

*HEMOGLOBINS, *TEMPERATURE, *CARBON dioxide, *COMPUTER simulation

Abstract

The functional properties of haemoglobin from the Mediterranean whale Balaenoptera physalus have been studied as functions of heterotropic effector concentration and temperature. Particular attention has been given to the effect of carbon dioxide and lactate since the animal is specialised for prolonged dives often in cold water. The molecular basis of the functional behaviour and in particular of the weak interaction with 2,3-diphosphoglycerate is discussed in the light of the primary structure and of computer modelling. On these bases, it is suggested that the A2 (Pro→Ala) substitution observed in the β chains of whale haemoglobin may be responsible for the displacement of the A helix known to be a key structural feature in haemoglobins that display an altered interaction with 2,3-diphosphoglycerate as compared with human haemoglobin. The functional and structural results, discussed in the light of a previous study on the haemoglobin from the Arctic whale Balaenoptera acutorostrata, give further insights into the regulatory mechanisms of the interactive effects of temperature, carbon dioxide and lactate. [Copyright &y& Elsevier]

Published

2003

126. Effects of salicylate on serotoninergic activities in rat inferior colliculus and auditory cortex

Author

Liu, Junxiu, Li, Xuepei, Wang, Lei, Dong, Yu, Han, Huiwan, and Liu, Guoquan

Subjects

*SEROTONIN, *INFERIOR colliculus, *AUDITORY cortex

Abstract

In vivo microdialysis offers a unique approach to monitor biochemical events related to brain function and metabolism, and has been used extensively in many systems to measure the release of endogenous transmitters and other neuroactive substances during normal and pathological conditions. The characterization of neurotransmitters’ changes induced by salicylate in the inferior colliculus (IC) and the auditory cortex (AC) may provide insight into the action of salicylate on the auditory system and, through this, provide a better understanding of neurological mechanism of salicylate-induced tinnitus. In the present study, the effect of salicylate on 5-HT system in IC and AC has been monitored by microdialysis in salicylate-induced tinnitus animal models. Glucose and lactate levels in IC and AC were significantly increased after application of salicylate (350 mg/kg, i.p.), indicating a salicylate-related increase in regional neuronal activity. The 5-HT level increased to a maximum of 268±27% basal level in IC 2 h after application and of 277±24% basal level in AC around 3 h after application. These data suggest that the increases of 5-HT levels in IC and AC may be involved in the tinnitus generation. [Copyright &y& Elsevier]

Published

2003

127. A high-affinity competitive inhibitor of type A botulinum neurotoxin protease activity

Author

Schmidt, James J. and Stafford, Robert G.

Subjects

*BOTULINUM toxin, *NEUROTOXIC agents

Abstract

The peptide N-acetyl-CRATKML-amide is an effective inhibitor of type A botulinum neurotoxin (BoNT A) protease activity [Schmidt et al., FEBS Lett. 435 (1998) 61–64]. To improve inhibitor binding, the peptide was modified by replacing cysteine with other sulfhydryl-containing compounds. Ten peptides were synthesized. One peptide adapted the structure of captopril to the binding requirements of BoNT A, but it was a weak inhibitor, suggesting that angiotensin-converting enzyme is not a good model for BoNT A inhibitor development. However, replacing cysteine with 2-mercapto-3-phenylpropionyl yielded a peptide with Ki of 330 nM, the best inhibitor of BoNT A protease activity reported to date. Additional modifications of the inhibitor revealed structural elements important for binding and supported our earlier findings that, with the exception of P1′ arginine, subsites on BoNT A are not highly specific for particular amino acid side chains. [Copyright &y& Elsevier]

Published

2002

128. Genetic susceptibility of mesocortical dopamine to stress determines liability to inhibition of mesoaccumbens dopamine and to behavioral ‘despair’ in a mouse model of depression

Author

Ventura, R., Cabib, S., and Puglisi-Allegra, S.

Subjects

*DOPAMINE, *PATHOLOGICAL psychology

Abstract

Clinical and preclinical research suggests a major role of mesocortical dopamine (DA) in psychopathology through regulation of subcortical, especially mesoaccumbens, DA functioning. In these experiments we demonstrate that the high vulnerability to stress-induced ‘despair’ and mesoaccumbens DA inhibition, exhibited by mice of the inbred strain C57BL/6 (C57) in a common animal model of depression, depends on their being highly susceptible to stress-induced mesocortical DA activation. Thus, C57 mice but not mice of the DBA/2 strain showed an extremely high level of immobility on their first experience with the forced swimming test (FST) as well as immediate and strong activation of mesocortical DA metabolism and inhibition of mesoaccumbens DA metabolism and release. In addition, the behavioral and the mesoaccumbens DA responses to FST in C57 mice were reduced and reversed, respectively, by bilateral mesocortical DA depletion. Finally, chronic treatment with the antidepressant clomipramine reduced immobility and eliminated both mesocortical DA activation and mesoaccumbens DA inhibition in response to FST.These results suggest that a genetically determined susceptibility to stress by the mesocortical DA system may favor the development of pathological behavioral responses through inhibition of subcortical DA transmission. [Copyright &y& Elsevier]

Published

2002

129. Suppression of sodium pump activity and an increase in the intracellular Ca2+ concentration by dexamethasone in acidotic mouse brain

Author

Namba, Chikara, Adachi, Naoto, Liu, Keyue, Yorozuya, Toshihiro, and Arai, Tatsuru

Subjects

*SODIUM/POTASSIUM ATPase, *ADENOSINE triphosphate

Abstract

The effects of dexamethasone on adenosine 5′-triphosphatase (ATPase) activity and the intracellular Ca2+ concentration ([Ca2+]i) were investigated in acidotic mouse brain. Dexamethasone (3 mg/kg, i.p.) or vehicle was administered 3 h before decapitation ischemia, and the brain concentration of adenosine 5′-triphosphate (ATP) was determined 0.5–2 min after ischemia. The effects of dexamethasone (0.3–3 mg/kg, i.p.) on Na+,K+-activated ATPase (Na+,K+-ATPase) and Ca2+-ATPase activities were evaluated at pH 7.4 and 6.8. Changes in [Ca2+]i in an acidic medium were determined in hippocampal slices by microfluorometry using rhod-2 acetoxymethyl ester as a Ca2+ marker, and the effects of dexamethasone (240 μg/l) was evaluated. Decapitation ischemia for 0.5 and 1 min reduced the brain ATP contents to 32% and 16% of the basal level, respectively. Dexamethasone slightly suppressed the extent of the decrease in the ATP level. Although dexamethasone did not affect Na+,K+-ATPase activity at pH 7.4, the activity was suppressed by dexamethasone (3 mg/kg) to 68% at pH 6.8. The activity of Ca2+-ATPase was not affected by dexamethasone at either pH 7.4 or pH 6.8. When the pH of the medium of the brain slices was changed from 7.4 to 6.8, almost no increase in [Ca2+]i was observed in the control group. The dexamethasone treatment increased [Ca2+]i in the CA1 field and dentate gyrus immediately after induction of the acidic medium, the effect being significant after 150 s. Because anaerobic glucose metabolism in the early stage of ischemia enhances intracellular lactic acidosis, the findings may suggest a mechanism for the aggravation of ischemic neuronal damage by glucocorticoids. [Copyright &y& Elsevier]

Published

2002

130. The interaction of β2-glycoprotein I domain V with chaperonin GroEL: The similarity with the domain V and membrane interaction.

Author

Gozu, Masayo, Hoshino, Masaru, Higurashi, Takashi, Kato, Hisao, and Goto, Yuji

Abstract

To clarify the mechanism of interaction between chaperonin GroEL and substrate proteins, we studied the conformational changes; of the fifth domain of human β2-glycoprotein I upon binding to GroEL. The fifth domain has a large flexible loop, containing several hydrophobic residues surrounded by positively charged residues, which has been proposed to be responsible for the binding of β2-glycoprotein I to negatively charged phospholipid membranes. The reduction by dithiothreitol of the three intramolecular disulfide bonds of the fifth domain was accelerated in the presence of stoichiometric amounts of GroEL, indicating that the fifth domain was destabilized upon interaction with GroEL. To clarify the GroEL-induced destabilization at the atomic level, we performed H/2H exchange of amide protons using heteronuclear NMR spectroscopy. The presence of GroEL promoted the H/2H exchange of most of the protected amide protons, suggesting that, although the flexible loop of the fifth domain is likely to be responsible for the initiation of binding to GroEL, the interaction with GroEL destabilizes the overall conformation of the fifth domain. [ABSTRACT FROM AUTHOR]

Published

2002

131. Amphioxus homologs of Go-coupled rhodopsin and peropsin having 11-cis- and all-trans-retinals as their chromophores

Author

Koyanagi, Mitsumasa, Terakita, Akihisa, Kubokawa, Kaoru, and Shichida, Yoshinori

Subjects

*BIOLOGICAL pigments, *G proteins

Abstract

Because of low contents in the native organs and failure of the expression in cultured cells, the chromophore configurations of the pigments in Go-coupled opsin and peropsin groups in the opsin family are unknown. Here we have succeeded in expression of the amphioxus homologs of these groups in HEK293s cells and found that they can be regenerated with 11-cis- and all-trans-retinals, respectively. Light isomerized the chromophores of these opsins into the all-trans and 11-cis forms, respectively. The results strongly suggest that the physiological function of peropsin would be a retinal photoisomerase, while 11-cis configuration is necessary for the Go-coupled opsin groups. [Copyright &y& Elsevier]

Published

2002

132. Preconditioned resistance to oxygen–glucose deprivation-induced cortical neuronal death: alterations in vesicular GABA and glutamate release

Author

Grabb, M.C., Lobner, D., Turetsky, D.M., and Choi, D.W.

Subjects

*CEREBRAL ischemia, *GABA

Abstract

Central neurons exposed to several types of sublethal stress, including ischemia, acquire resistance to injury induced by subsequent ischemic insults, a phenomenon called ischemic preconditioning. We modeled this phenomenon in vitro, utilizing exposure to 45 mM KCl to reduce the vulnerability of cultured murine cortical neurons to subsequent oxygen–glucose deprivation. Twenty-four hours after preconditioning, cultures exhibited enhanced depolarization-induced, tetanus toxin-sensitive GABA release and a modest decrease in glutamate release. Total cellular GABA levels were unaltered. Inhibition of GABA degradation with the GABA transaminase inhibitor (±)-γ-vinyl GABA, or addition of low levels of GABA, muscimol, or chlormethiazole to the bathing medium, mimicked the neuroprotective effect of preconditioning against oxygen–glucose deprivation-induced death. However, neuronal death was enhanced by higher levels of these manipulations, as well as by prior selective destruction of GABAergic neurons by kainate. Finally, selective blockade of GABAA receptors during oxygen–glucose deprivation or removal of GABAergic neurons eliminated the neuroprotective effects of prior preconditioning.Taken together, these data predict that presynaptic alterations, specifically enhanced GABA release together with reduced glutamate release, may be important mediators of ischemic preconditioning, but suggest caution in regard to interventions aimed at increasing GABAA receptor activation. [Copyright &y& Elsevier]

Published

2002

133. Characterization of a novel human UDP-GalNAc transferase, pp-GalNAc-T101<FN ID="FN1"><NO>1</NO>The nucleotide sequence of human pp-GalNAc-T10 reported in this paper has been deposited in the DDBJ/EMBL/GenBank databases with accession number AB078145.</FN>

Author

Cheng, Lamei, Tachibana, Kouichi, Zhang, Yan, Guo, Jian-ming, Kahori Tachibana, Kahori, Kameyama, Akihiko, Wang, Han, Hiruma, Toru, Iwasaki, Hiroko, Togayachi, Akira, Kudo, Takashi, and Narimatsu, Hisashi

Subjects

*MOLECULAR cloning, *POLYMERASE chain reaction

Abstract

A novel member of the human UDP-N-acetyl-D-galactosamine:polypeptide N-acetylgalactosaminyltransferase (pp-GalNAc-T) gene family was cloned as a homolog of human pp-GalNAc-T7, and designated pp-GalNAc-T10. pp-GalNAc-T10 transcript was found in the small intestine, stomach, pancreas, ovary, thyroid gland and spleen. In a polypeptide GalNAc-transfer assay, recombinant pp-GalNAc-T10 transferred GalNAc onto a panel of mucin-derived peptide substrates. Furthermore, pp-GalNAc-T10 demonstrated strong transferase activity with glycopeptide substrates. [Copyright &y& Elsevier]

Published

2002

134. Unilateral infusion of a dopamine transporter antisense into the substantia nigra protects against MDMA-induced serotonergic deficits in the ipsilateral striatum

Author

Kanthasamy, A., Sprague, J.E., Shotwell, J.R., and Nichols, D.E.

Subjects

*ANTISENSE nucleic acids, *OLIGONUCLEOTIDES, *TRYPTOPHAN, *DOPAMINE

Abstract

The present study was designed to elucidate the consequences of antisense oligonucleotide-mediated knockdown of striatal dopamine reuptake transporters on 3,4-methylenedioxymethamphetamine (MDMA)-induced neurotoxicity. Antisense oligonucleotide complementary to the mRNA translational start site of the rat dopamine transporter was delivered by constant (7 days) intranigral infusion with an osmotic minipump. Delivery of the antisense oligonucleotide by this method resulted in a 70% reduction in the density of the dopamine transporter in the ipsilateral striatum, as measured by [3H]mazindol binding. The effect of this transporter knockdown on MDMA-induced serotonergic neurotoxicity was then examined. MDMA (2×20 mg/kg, s.c., given 12 h apart) administered to control rats produced hyperthermia following the first dose and led to a 45–50% reduction in striatal serotonin, 5-hydroxyindoleacetic acid, and serotonin reuptake transporter density 1 week after the second dose. Conversely, in antisense-, but not missense-treated rats, a significant attenuation of MDMA-induced neurotoxicity was observed only in the ipsilateral striatum. The hyperthermic response elicited by MDMA was not altered by prior administration of antisense. In vivo microdialysis revealed that the antisense treatment attenuated MDMA-induced dopamine release in the ipsilateral striatum.These results suggest that the dopamine transporter plays an essential role in the neurodegeneration induced by MDMA, and provides additional support for the hypothesis that extracellular dopamine is involved in the neurotoxic process, at least in the striatum. [Copyright &y& Elsevier]

Published

2002

135. The role of helix stabilizing residues in GCN4 basic region folding and DNA binding.

Author

Hollenbeck, Jessica J., McClain, Diana L., and Oakley, Martha G.

Abstract

Basic region leucine zipper (bZip) proteins contain a bipartite DNA-binding motif consisting of a coiled-coil leucine zipper dimerization domain and a highly charged basic region that directly contacts DNA. The basic region is largely unfolded in the absence of DNA, but adopts a helical conformation upon DNA binding. Although a coil → helix transition is entropically unfavorable, this conformational change positions the DNA-binding residues appropriately for sequence-specific interactions with DNA. The N-terminal residues of the GCN4 DNA-binding domain, DPAAL, make no DNA contacts and are not part of the conserved basic region, but are nonetheless important for DNA binding. Asp and Pro are often found at the N-termini of α-helices, and such N-capping motifs can stabilize α-helical structure. In the present study, we investigate whether these two residues serve to stabilize a helical conformation in the GCN4 basic region, lowering the energetic cost for DNA binding. Our results suggest that the presence of these residues contributes significantly to helical structure and to the DNA-binding ability of the basic region in the absence of the leucine zipper. Similar helix-capping motifs are found in approximately half of all bZip domains, and the implications of these findings for in vivo protein function are discussed. [ABSTRACT FROM AUTHOR]

Published

2002

136. Involvement of the medial prefrontal cortex in mediating behavioural responses to odour cues rather than olfactory recognition memory

Author

Broad, K.D., Hinton, M.R., Keverne, E.B., and Kendrick, K.M.

Subjects

*MEMORY, *SMELL, *DOPAMINE

Abstract

Sheep form an olfactory recognition memory for their lambs within 2 h of parturition and will subsequently reject the approaches of any strange lamb and protest vocally. In this study we report that following olfactory memory formation, ewes exposed to either their own or a strange lamb show c-fos mRNA expression in the medial frontal cortex, although levels of expression in the pyramidal output cell layer V were significantly higher in ewes that rejected strange lambs. Reversibly inactivating this region by the retrodialysis of the anaesthetic tetracaine before birth reduced aggressive motor responses towards lambs but not protest vocalisations. Similar treatment during the critical period for olfactory memory formation and lamb recognition (0–4 h post-partum) had no effect on ewes maternal behaviour towards their own lambs. It did, however, prevent the normal selective expression of aggressive rejection, and reduced protest vocalisation behaviours directed towards strange lambs. These rejection behaviours did appear 1 h after the termination of tetracaine infusions despite the ewes not being given the opportunity to interact with their own lambs during this time. Therefore, tetracaine blockade of the medial frontal cortex prevents animals from responding with motor aggression, but not vocal aggression, to odour cues from strange lambs, but has no effect on the formation of an olfactory recognition memory for their own lambs. Both pre- and post-partum aggressive rejection of strange lambs was associated with increased concentrations of dopamine, serotonin, glutamate and GABA. When these behaviours were inhibited by the tetracaine infusions, extracellular concentrations of these neurotransmitters were all increased by the anaesthetic but did not change in response to lambs. These findings suggest that a functional medial frontal cortex is not required for the formation of an olfactory recognition memory or for mediating pro-active maternal behaviours. It is however required for the mediation of motor but not vocal aspects of aggressive rejection responses directed towards aversive odour cues from strange lambs. [Copyright &y& Elsevier]

Published

2002

137. Regulation of medial prefrontal cortex dopamine by α-amino-3-hydroxy-5-methylisoxazole-4-propionate/kainate receptors

Author

Wu, W.-R., Li, N., and Sorg, B.A.

Subjects

*CEREBROSPINAL fluid, *DOPAMINE receptors, *COCAINE

Abstract

In the medial prefrontal cortex, repeated cocaine produces tolerance of the extracellular dopamine response to subsequent cocaine injection. These studies characterized the influence of α-amino-3-hydroxy-5-methylisoxazole-4-propionate/kainate receptors on the medial prefrontal cortex dopamine response to acute cocaine, amphetamine and potassium chloride as a first step to assess whether these receptor subtypes may be candidates for mediating dopamine tolerance after repeated cocaine. Local infusion of 10 μM 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX) produced an approximate 40% increase in dopamine levels in the medial prefrontal cortex, while a 30 μM dose did not alter basal levels infused over a 3-h period. Thus, 30 μM CNQX was chosen for the remaining experiments, and was infused for 1 h prior to and during all in vivo treatments. Local medial prefrontal cortex infusion of the 30 μM dose blocked the small increase in dopamine levels elicited by systemic saline injection (maximum of 26%), as well as the much larger increase in response to acute cocaine injection (maximum of 340%). Local infusion of D-amphetamine (3 and 30 μM) through the probe increased dopamine to 300 and 600% of basal levels, respectively. Co-infusion of CNQX partially blocked the response for the first 40 min, but dopamine levels recovered by 60 min later. Local infusion of 100 mM potassium chloride elicited a 600% increase in dopamine levels, which was attenuated approximately 50% by CNQX co-infusion. Potassium-stimulated release of dopamine was also measured in vitro in medial prefrontal cortical and striatal tissue. By 30 s after potassium addition, dopamine levels increased to 800% above baseline in the medial prefrontal cortex, and this increase was blocked by the presence of 30 μM CNQX. In contrast, potassium-stimulated dopamine release in striatal tissue was approximately 250% above basal levels, with no effect of CNQX on dopamine release. Locomotor behavior collected during dialysis experiments demonstrated that increased activity induced by local infusion of potassium chloride was severely attenuated by co-infusion of 30 μM CNQX, while no effects of this drug were found for cocaine-elicited behavior. These results suggest a potent influence of glutamate via α-amino-3-hydroxy-5-methylisoxazole-4-propionate/kainate receptors on extracellular dopamine in the medial prefrontal cortex, and these receptors may regulate dopamine release through a presynaptic mechanism.The findings may help elucidate the role of medial prefrontal cortex dopamine–glutamate interactions in drug abuse and stress- and drug-precipitated psychosis. [Copyright &y& Elsevier]

Published

2002

138. Effects of neonatal handling on basal and stress-induced monoamine levels in the male and female rat brain

Author

Papaioannou, A., Dafni, U., Alikaridis, F., Bolaris, S., and Stylianopoulou, F.

Subjects

*BRAIN, *PHYSIOLOGICAL stress

Abstract

Neonatal handling has pervasive effects on the rat brain leading to increased ability to cope with and adapt to stressful stimuli. We determined the effects of neonatal handling on the dopaminergic and serotonergic system, in the male and female rat brain, under basal conditions before and after puberty and after short- and long-term forced swimming stress.Exposure of animals to neonatal handling resulted in sex-dependent changes in the concentration and turnover of monoamines in the different brain areas. In the prepubertal brain, the effect of neonatal handling was manifested as an increase in dopamine turnover in the females, particularly in the hypothalamus, an increase in serotonin levels and a decrease in its turnover in all three brain regions examined of both males and females. Certain of the handling-induced effects observed in the prepubertal brain were reversed in the postpubertal animals. Thus, in the postpubertal brain, the handling-induced changes in serotonin levels and its turnover observed in both sexes before puberty were abolished. On the other hand, the handling-induced increase in hypothalamic dopamine turnover was maintained. After exposure to short-term stress, the effect of handling was manifested on one hand as decreased striatal dopamine levels in the females, and decreased dopamine turnover in the hypothalamus of both males and females, and on the other, as increased serotonin levels in the hypothalamus. After exposure to long-term stress, handled females had decreased dopamine turnover in the hypothalamus and the striatum, but there was no effect of handling on the serotonergic system.Our results provide some neurobiological evidence supporting the determinant role of the mother–infant relationship in the development of psychopathology. Neonatal handling, which modifies normal mother–pup interactions, results in alterations in brain dopaminergic and serotonergic systems, both of which are involved in the etiopathogenesis of major psychoses. Exposure to either short- or long-term stress in adult life results in sex-dependent changes in brain monoamines, which are affected by handling thus making coping more efficient and rendering the stressful stimulus less noxious. [Copyright &y& Elsevier]

Published

2002

139. Maltooligosaccharide disproportionation reaction: an intrinsic property of amylosucrase from Neisseria polysaccharea

Author

Albenne, Cécile, Skov, Lars K., Mirza, Osman, Gajhede, Michael, Potocki-Véronèse, Gabrielle, Monsan, Pierre, and Remaud-Simeon, Magali

Subjects

*GLYCOSYLTRANSFERASES, *MALTOSE

Abstract

Amylosucrase from Neisseria polysaccharea (AS) is a remarkable transglycosidase of family 13 of the glycoside hydrolases that catalyses the synthesis of an amylose-like polymer from sucrose and is always described as a sucrose-specific enzyme. Here, we demonstrate for the first time the ability of pure AS to catalyse the disproportionation of maltooligosaccharides by cleaving the α-1,4 linkage at the non-reducing end of a maltooligosaccharide donor and transferring the glucosyl unit to the non-reducing end of another maltooligosaccharide acceptor. Surprisingly, maltose, maltotriose and maltotetraose are very poor glucosyl donors whereas longer maltooligosaccharides are even more efficient glucosyl donors than sucrose. At least five glucose units are required for efficient transglucosylation, suggesting the existence of strong binding subsites, far from the sucrose binding site, at position +4 and above. [Copyright &y& Elsevier]

Published

2002

140. Grafts of fetal septal cells after cholinergic immunotoxic denervation of the hippocampus: a functional dissociation between dorsal and ventral implantation sites

Author

Cassel, J.-C., Gaurivaud, M., Lazarus, C., Bertrand, F., Galani, R., and Jeltsch, H.

Subjects

*DENERVATION, *HIPPOCAMPUS (Brain)

Abstract

Three-month-old Long–Evans rats were subjected to intraseptal infusions of 0.8 μg of 192 IgG–saporin followed, 2 weeks later, by intrahippocampal suspension grafts containing fetal cells from the medial septum and the diagonal band of Broca. The suspensions were implanted in the dorsal or the ventral hippocampus. Sham-operated and lesion-only rats were used as controls. Between 18 and 32 weeks after grafting, all rats were tested in a water maze (using protocols placing emphasis on reference memory or on working memory) and an eight-arm radial maze. The lesion produced extensive cholinergic denervation of the hippocampus, as evidenced by reduced acetylcholinesterase-positivity and acetylcholine content. Depending upon their implantation site, the grafts restored an acetylcholinesterase-positive reinnervation pattern in either the dorsal or the ventral hippocampus. Nevertheless, the grafts failed to normalize the concentration of acetylcholine in either region. The cholinergic lesion impaired working memory performance in both the water maze and the radial maze. To a limited degree, reference memory was also altered. Grafts placed in the ventral hippocampus had no significant behavioral effect, whereas those placed in the dorsal hippocampus normalized working memory performance in the water maze.Our data show that infusion of 192 IgG–saporin into the septal region deprived the hippocampus of its cholinergic innervation and altered spatial working memory more consistently than spatial reference memory. Although the cholinergic nature of the graft-induced reinnervation remains to be established more clearly, these results further support the idea of a functional dissociation between the dorsal and the ventral hippocampus, the former being preferentially involved in spatial memory. [Copyright &y& Elsevier]

Published

2002

141. 3β-Hydroxysteroid dehydrogenase expression in rat spinal cord

Author

Coirini, H., Gouézou, M., Liere, P., Delespierre, B., Pianos, A., Eychenne, B., Schumacher, M., and Guennoun, R.

Subjects

*SPINAL cord, *DEHYDROGENASES, *CELLS

Abstract

In adult male rats, 3β-hydroxysteroid dehydrogenase/Δ5-Δ4-isomerase (3β-HSD) expressing cells were identified in the spinal cord from the cervical to the sacral segments. An in situ hybridization study, using an oligonucleotide common to the four known isoforms of rat 3β-HSD, revealed its mRNA in gray matter. Measurements of optical densities in autoradiograms showed the following regional distribution: dorsal horn (layers I–III)>central canal (layer X)≥ventral horn (layers VIII–IX)>ventral funiculus=lateral funiculus. At the cellular level, the number of grains was higher on the large motoneurons than on small neurons of the dorsal horn, but the grain density per cell was similar. Further evidence for the expression of 3β-HSD in the spinal cord was obtained by western blot analysis, which revealed an immunoreactive protein of &ap;45 kDa in the dorsal and ventral parts of the spinal cord. Castration and adrenalectomy did not influence the expression of 3β-HSD mRNA and protein. Gas chromatography/mass spectrometry measurements showed higher levels of pregnenolone and progesterone in the spinal cord than in the plasma. After castration and adrenalectomy, their levels remained elevated in the spinal cord, suggesting that these neurosteroids may be synthesized locally.The wide distribution of 3β-HSD, and the high levels of pregnenolone and progesterone in the spinal cord even after castration and adrenalectomy, strongly suggest a potential endogenous production of progesterone and an important signalling function of this steroid in the spinal cord. [Copyright &y& Elsevier]

Published

2002

142. Interactions among adenosine deaminase, adenosine A1 receptors and dopamine D1 receptors in stably cotransfected fibroblast cells and neurons

Author

Torvinen, M., Ginés, S., Hillion, J., Latini, S., Canals, M., Ciruela, F., Bordoni, F., Staines, W., Pedata, F., Agnati, L.F., Lluis, C., Franco, R., Ferré, S., and Fuxe, K.

Subjects

*ADENOSINE deaminase, *DOPAMINE receptors, *FIBROBLASTS

Abstract

The role of adenosine deaminase in the interactions between adenosine A1 and dopamine D1 receptors was studied in a mouse fibroblast cell line stably cotransfected with human D1 receptor and A1 receptor cDNAs (A1D1 cells). Confocal laser microscopy analysis showed a high degree of adenosine deaminase immunoreactivity on the membrane of the A1D1 cells but not of the D1 cells (only cotransfected with human D1 receptor cDNAs). In double immunolabelling experiments in A1D1 cells and cortical neurons a marked overlap in the distribution of the A1 receptor and adenosine deaminase immunoreactivities and of the D1 receptor and adenosine deaminase immunoreactivities was found. Quantitative analysis of A1D1 cells showed that adenosine deaminase immunoreactivity to a large extent colocalizes with A1 and D1 receptor immunoreactivity, respectively. The A1 receptor agonist caused in A1D1 cells and in cortical neurons coaggregation of A1 receptors and adenosine deaminase, and of D1 receptors and adenosine deaminase. The A1 receptor agonist-induced aggregation was blocked by R-deoxycoformycin, an irreversible adenosine deaminase inhibitor. The competitive binding experiments with the D1 receptor antagonist [3H]SCH-23390 showed that the D1 receptors had a better fit for two binding sites for dopamine, and treatment with the A1 receptor agonist produced a disappearance of the high-affinity site for dopamine at the D1 receptor. R-Deoxycoformycin treatment, which has previously been shown to block the interaction between adenosine deaminase and A1 receptors, and which is crucial for the high-affinity state of the A1 receptor, also blocked the A1 receptor agonist-induced loss of high-affinity D1 receptor binding.The conclusion of the present studies is that the high-affinity state of the A1 receptor is essential for the A1 receptor-mediated antagonistic modulation of D1 receptors and for the A1 receptor-induced coaggregates of A1 and adenosine deaminase, and of D1 and adenosine deaminase. Thus, the confocal experiments indicate that both A1 and D1 receptors form agonist-regulated clusters with adenosine deaminase, where the presence of a structurally intact adenosine deaminase bound to A1 receptors is important for the A1–D1 receptor–receptor interaction at the level of the D1 receptor recognition. [Copyright &y& Elsevier]

Published

2002

143. Therapeutic effects of astrocytes expressing both tyrosine hydroxylase and brain-derived neurotrophic factor on a rat model of Parkinson’s disease

Author

Wang, Z.H., Ji, Y., Shan, W., Zeng, B., Raksadawan, N., Pastores, G.M., Wisniewski, T., and Kolodny, E.H.

Subjects

*TYROSINE, *ASTROCYTES

Abstract

Tyrosine hydroxylase (TH) and brain-derived neurotrophic factor (BDNF), expressed in normal astrocytes, were used in combination for the treatment of Parkinson’s disease (PD) symptoms in a rat model. Normal neonatal rat astrocytes were co-transfected with a vector expressing BDNF (AAVBDNF) and a retroviral vector expressing TH (termed TH-BDNF-DA+ cells), and then implanted into the striatum of PD rats induced by 6-hydroxydopamine. TH-BDNF-DA+ cells compensated for a severe insufficiency of endogenous dopaminergic neurons in the PD rats, resulting in a significant improvement of PD symptoms. The decrease in the rotational rate of PD rats implanted with TH-BDNF-DA+ cells was more marked than that in PD rats implanted with normal astrocytes expressing either TH or BDNF alone (termed TH+ and BDNF+ cells, P<0.01 and 0.001, respectively), and suggested a synergistic effect between TH and BDNF. In contrast, the rotational rate was not altered from the baseline in PD rats without treatment or implanted with parental rat astrocytes alone (P>0.05). BDNF protected the dopaminergic neurons from apoptosis induced by 6-hydroxydopamine, and significantly increased the long-term survival of TH-positive cells in the striatum.Our data indicate that the combined use of TH and BDNF has a synergistic therapeutic effect, and is more efficient for the treatment of PD than a single gene therapy using either TH or BDNF alone. [Copyright &y& Elsevier]

Published

2002

144. Facilitation of learning and modulation of frontal cortex acetylcholine by ventral pallidal injection of heparin glucosaminoglycan

Author

De Souza Silva, M.A., Jezek, K., Weth, K., Müller, H.W., Huston, J.P., Brandao, M.L., and Hasenöhrl, R.U.

Subjects

*HEPARIN, *ACETYLCHOLINE, *ANALYSIS of variance, *FRONTAL lobe

Abstract

We examined the effects of heparin on learning and frontal cortex acetylcholine parameters following injection of the glucosaminoglycan into the ventral pallidum. In Experiment 1, possible mnemoactive effects of intrapallidal heparin injection were assessed. Rats with chronically implanted cannulae were administered heparin (0.1, 1.0, 10 ng) or vehicle (0.5 μl) and were tested on a one-trial step-through avoidance task. Two retention tests were carried out in each animal, one at 1.5 h after training to measure short-term memory and another at 24 h to measure long-term memory. Post-trial intrapallidal injection of 1.0 ng heparin improved both short- and long-term retention of the task, whereas the lower and the higher dose of the glucosaminoglycan had no effect. When the effective dose of heparin was injected 5 h, rather than immediately after training, it no longer facilitated long-term retention of the conditioned avoidance response. In Experiment 2, the effects of ventral pallidal heparin injection on frontal cortex acetylcholine and choline concentrations were investigated with in vivo microdialysis in anaesthetized rats. Heparin, administered in the dose of 1.0 ng, which was effective in facilitating avoidance performance, produced a delayed increase in cortical acetylcholine levels ipsi- and contralaterally to the side of intrabasalis injection, resembling the known neurochemical effects obtained for another glycosaminoglycan, chondroitin sulfate, which recently was shown to facilitate inhibitory avoidance learning and to increase frontal cortex acetylcholine.The present findings indicate that heparin, like other extracellular matrix proteoglycans, can exert beneficial effects on memory and strengthen the presumptive relationship between such promnestic effects of proteoglycans and basal forebrain cholinergic mechanisms. The data are discussed with respect to the presumed roles of matrix molecules in extrasynaptic volume transmission and in the ‘cross-talk’ between synapses. [Copyright &y& Elsevier]

Published

2002

145. Inhibition of hepatitis C virus NS3 protease by peptides derived from complementarity-determining regions (CDRs) of the monoclonal antibody 8D4: tolerance of a CDR peptide to conformational changes of a target

Author

Tsumoto, Kouhei, Misawa, Satoru, Ohba, Yoichi, Ueno, Takamasa, Hayashi, Hideya, Kasai, Nobuhiro, Watanabe, Hideki, Asano, Ryutaro, and Kumagai, Izumi

Subjects

*PEPTIDES, *HEPATITIS C virus, *HIGH performance liquid chromatography

Abstract

We have synthesized and characterized peptides derived from complementarity-determining regions (CDRs) of 8D4, a mouse monoclonal antibody against NS3 protease domain of hepatitis C virus. 8D4 inhibits enzymatic activity without its cofactor, NS4A peptide. One of the synthetic peptides derived from CDRs, CDR1 of the heavy-chain (CDR-H1) peptide strongly inhibited NS3 protease activity competitively in the absence of NS4A and non-competitively in the presence of NS4A. Moreover, cyclic CDR-H1 peptides bridged by disulfide inhibited NS3 protease more potently. The chain length of the CDR-H1 peptide is critical for strong inhibition, even when the peptide is circularized. This finding suggests the importance of peptide conformation. In contrast to a cognate antibody molecule, CDR-derived peptides may provide good ligands for target molecules by having a tolerance to conformational changes of the targets caused by cofactor binding or mutation. [Copyright &y& Elsevier]

Published

2002

146. Feeding-induced decrease in extracellular glutamate level in the rat nucleus accumbens: dependence on glutamate uptake

Author

Saulskaya, N.B. and Mikhailova, M.O.

Subjects

*CEREBROSPINAL fluid, *CHROMATOGRAPHIC analysis, *ELECTROCHEMICAL analysis

Abstract

In vivo microdialysis combined with high-performance liquid chromatography and electrochemical detection was used to monitor extracellular glutamate levels in the medial nucleus accumbens of Sprague–Dawley rats during their feeding behaviour. Consumption of a palatable new diet or a diet to which rats were previously exposed caused a decrease in extracellular level of glutamate in the nucleus accumbens during and after feeding. The presentation of an inedible object (a piece of rubber) instead of the expected food caused a marked increase in extracellular glutamate levels. In contrast, if the piece of rubber was presented to rats that did not expect food delivery, the extracellular level of glutamate remained unchanged during the rubber presentation. The feeding-induced decrease in the extracellular glutamate level did not depend on food deprivation and was completely prevented by intraaccumbal infusions through the dialysis probe of 10 mM D,L-threo-β-hydroxyaspartate (a glutamate uptake inhibitor). Intraaccumbal infusions of 10 μM S-(−)-raclopride L-tartrate (a D2/D3 dopamine receptor antagonist) or 1 μM tetrodotoxin (a voltage-dependent Na+ channel blocker) also completely reversed the decrease in extracellular glutamate level in response to food intake. The D1/D5 dopamine receptor antagonist SCH-23390 (10 μM) administered into the nucleus accumbens had no significant effect on the feeding-induced decrease in extracellular glutamate level.From the data obtained we suggest that the decrease in the extracellular level of glutamate in the medial nucleus accumbens in response to feeding appears to arise from a temporal increase in glutamate uptake that is probably operated by dopamine inputs to the nucleus accumbens via D2/D3 receptors. Our findings also suggest that the dissociation between the expected biological value of a presented object and the reality might be an important determinant for regulation of glutamate release in this brain area during feeding behaviour. [Copyright &y& Elsevier]

Published

2002

147. Isolation rearing in the rat disrupts the hippocampal response to stress

Author

Muchimapura, S., Fulford, A.J., Mason, R., and Marsden, C.A.

Subjects

*SCHIZOPHRENIA, *AMYGDALOID body, *HIPPOCAMPUS (Brain)

Abstract

Both human schizophrenia and the effects of isolation rearing in rats produce deficits in hippocampal and cortical functioning. This study was concerned with identifying changes associated with altered neuronal function in the rat hippocampus following isolation rearing. Rats were isolated from weaning at 21 days postnatal for 6 weeks and the hippocampal sensitivity to isolation rearing and stress were studied using c-fos immunohistochemistry and in vivo microdialysis. Isolation rearing altered neuronal activity measured by Fos-like immunoreactivity in the specific brain areas as measured by either increased or reduced expression. Basal neuronal activity in the ventral CA1 hippocampus in isolation-reared rats was notably higher compared to group-reared rats but markedly lower Fos-like immunoreactivity was found in the central and basolateral nuclei of the amygdala. Exposure to stress produced differential effects on neuronal activity in isolation-reared rats between the dorsal and ventral hippocampus, with increased Fos-like immunoreactivity in the dorsal hippocampus but lower Fos-like immunoreactivity in the ventral hippocampus compared to group-reared rats. These results indicate that isolation rearing may alter the relationship between hippocampal neuronal function in the dorsal and ventral hippocampus. An in vivo microdialysis study showed that systemically administered parachloroamphetamine (2.5 mg/kg, i.p.) enhanced extracellular 5-hydroxytryptamine (5-HT) in the dorsal hippocampus in group-reared but not in isolation-reared rats. Restraint stress had no effect on hippocampal extracellular 5-HT in group-reared rats but reduced levels in isolation-reared rats during the period of restraint. Inescapable mild footshock produced a marked increase in extracellular hippocampal 5-HT in group-reared but not isolation-reared rats.Overall the results provide extensive evidence that isolation rearing alters presynaptic 5-HT hippocampal function and that the neuronal response to stress is altered by isolation. Isolation rearing in the rat alters hippocampal function, including the serotonergic system, leading to changes in neurotransmitter systems in other brain areas. These changes may model aspects of human neurodevelopmental disorders such as schizophrenia. [Copyright &y& Elsevier]

Published

2002

148. The neuropeptide Y monomer in solution is not folded in the pancreatic-polypeptide fold.

Author

Bettio, Andrea, Dinger, Michaela C., and Beck-Sickinger, Annette G.

Abstract

Fluorescence-labelled analogs of NPY, a 36-amino acid peptide amide, were synthesized by solid-phase peptide synthesis and used for fluorescence-resonance energy transfer studies to investigate the conformation. Energy-transfer efficiency measurements in different media at the concentration of 10 μM are in agreement with a model of the NPY structure proposed by NMR studies (performed at millimolar concentration) in which the C-terminal part of the molecule adopts an α-helical conformation while the N-terminal part is flexible. According to this model, the α-helix is stabilized by intermolecular hydrophobic interactions because of the formation of dimers. The decrease of the peptide concentration causes a shift of the dimerization equilibrium toward the monomeric form. Energy-transfer efficiency measurements performed at lower concentrations do not support the hypothesis of the folding back of the N-terminal tail onto the C-terminal α-helix to yield the so-called 'PP-fold' conformation. This structure is observed in the crystal structure of avian pancreatic polypeptide, a member of the NPY peptide hormone family, and it has been considered to be the bioactive one. Our results complete the structural characterization of NPY in solution at concentration ranges in which NMR experiments are not feasible. Furthermore, these results open the way to study the conformation of the receptor-bound ligand. [ABSTRACT FROM AUTHOR]

Published

2002

149. Cloning and characterization of Streptomyces galilaeus aclacinomycins polyketide synthase (PKS) cluster

Author

Räty, Kaj, Kantola, Jaana, Hautala, Anne, Hakala, Juha, Ylihonko, Kristiina, and Mäntsälä, Pekka

Subjects

*POLYKETIDES, *LIQUID chromatography

Abstract

We have cloned and sequenced polyketide synthase (PKS) genes from the aclacinomycin producer Streptomyces galilaeus ATCC 31,615. The sequenced 13.5-kb region contained 13 complete genes. Their organization as well as their protein sequences showed high similarity to those of other type II PKS genes. The continuous region included the genes for the minimal PKS, consisting of ketosynthase I (aknB), ketosynthase II (aknC), and acyl carrier protein (aknD). These were followed by the daunomycin dpsC and dpsD homologues (aknE2 and F, respectively), which are rare in type II PKS clusters. They are associated with the unusual starter unit, propionate, used in the biosynthesis of aklavinone, a common precursor of aclacinomycin and daunomycin. Accordingly, when aclacinomycins minimal PKS genes were substituted for those of nogalamycin in the plasmid carrying genes for auramycinone biosynthesis, aklavinone was produced in the heterologous hosts. In addition to the minimal PKS, the cloned region included the PKS genes for polyketide ketoreductase (aknA), aromatase (aknE1) and oxygenase (aknX), as well as genes putatively encoding an aklanonic acid methyl transferase (aknG) and an aklanonic acid methyl ester cyclase (aknH) for post-polyketide steps were found. Moreover, the region carried genes for an activator (aknI), a glycosyl transferase (aknK) and an epimerase (aknL) taking part in deoxysugar biosynthesis. [Copyright &y& Elsevier]

Published

2002

150. Solid-phase synthesis of new peptide–arene hybrids from N-TCP amino acids

Author

Planas, Marta, Cros, Esther, Rodrıguez, Ricard-Aleix, Ferre, Rafael, and Bardajı, Eduard

Subjects

*SOLID-phase synthesis, *MACROCYCLIC compounds, *PEPTIDES

Abstract

New linear and macrocyclic arene–peptide hybrids may be synthesized from N-tetrachlorophthaloyl protected amino acids through mild phthalimide opening by 1,3-diaminopropane. [Copyright &y& Elsevier]

Published

2002