UMLS:C1519176 - FACTA Search

Gene/Protein Disease Symptom Drug Enzyme Compound
Pivot Concepts: Target Concepts:

Query: UMLS:C1519176 (PSA)
5,490 document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)

Polyclonal rabbit antiserum to the Triton X-114 phase material of Leishmania major, which comprises the surface and internal integral membrane proteins of the parasite, was used to screen a lambda gt11 genomic expression library. A recombinant clone producing a Mr 123,000 beta-galactosidase fusion protein was isolated. Antibodies affinity-purified on this fusion protein recognized a complex of three surface-oriented proteins of promastigotes of L. major of Mr 94,000, 90,000, and 80,000 that we have termed the promastigote surface Ag 2 (PSA-2) complex. The DNA sequence of the insert in this clone predicted the 3' end of an open reading frame encoding a hydrophobic C-terminus. The inferred C-terminal sequence was suggestive of a glycosylphosphatidyl-inositol membrane anchoring mechanism. Phosphatidylinositol-specific phospholipase C treatment of the native PSA-2 proteins caused a shift in their electrophoretic mobility with an apparent reduction in the molecular weight of the PSA-2 complex. After phospholipase C treatment these proteins also displayed the cryptic cross-reacting determinant recognized by antibodies to the Trypanosoma brucei variant surface Ag. Moreover, PSA-2, which previously partitioned in the detergent phase after Triton X-114 phase separation, became water-soluble after phospholipase C treatment. Immunoprecipitation of the PSA-2 proteins with sera directed to lectin-binding proteins indicated that these polypeptides may be differentially glycosylated. Finally, these PSA-2 proteins were recognized by sera from some patients with cutaneous leishmaniasis.
...
PMID:The PSA-2 glycoprotein complex of Leishmania major is a glycosylphosphatidylinositol-linked promastigote surface antigen. 259 73

Measurements of the magnetic field dependence of the longitudinal magnetic relaxation rates (NMRD profiles) of solvent protons and deuterons led to the discovery of two classes of solvent binding sites in Ca2+-Mn2+-concanavalin A (CMPL) [Koenig, S. H., Brown, R. D., III, & Brewer, C. F. (1985) Biochemistry (second of three papers in this issue)]. In this paper, we compare proton and deuteron NMRD profiles of Ca2+-Mn2+-lentil lectin (CMLcH) and Ca2+-Mn2+-pea lectin (CMPSA) with those of CMPL. All three metalloproteins are D-mannose/D-glucose-specific lectins that have a high degree of structural similarity and require the metal ions for their biological activities. We have developed a method for the preparation of fully active metal ion derivatives of lentil lectin (LcH) and pea lectin (PSA), including the diamagnetic derivatives Ca2+-Zn2+-LcH and Ca2+-Zn2+-PSA [Bhattacharyya, L., Brewer, C. F., Brown, R. D., III, & Koenig, S. H.(1984) Biochem. Biophys. Res. Commun. 124, 857-862]. The behavior of these two lectins with regard to their NMRD profiles is essentially identical, for both the paramagnetic and diamagnetic forms. Together with CMPL, all three lectins have a common paramagnetic contribution with a negative temperature dependence of the rates, while CMPL contributes an additional component with a positive temperature dependence. The common contribution derives from the class of fast exchanging water molecules observed in the proton NMRD profile of CMPL (Koenig et al., 1985); their protons are calculated to be relatively remote from the Mn2+ ions (4.4 A for CMPL and 5.5 A for LcH and PSA).(ABSTRACT TRUNCATED AT 250 WORDS)
...
PMID:Proton and deuteron nuclear magnetic relaxation dispersion studies of Ca2+-Mn2+-lentil lectin and Ca2+-Mn2+-pea lectin: evidence for a site of solvent exchange in common with concanavalin A. 407 70

Antibodies raised against a Leishmania major recombinant promastigote surface antigen 2 (PSA-2) fragment recognized three major polypeptides of approximate M(r) 96,000, 80,000 and 50,000 in promastigotes of three Israeli isolates of L. major including the cloned line LRC-L137-V121, but detected a different array of polypeptides in other L. major isolates. The pattern was different both in number of polypeptides detected and their molecular weight. The antibodies to L. major PSA-2 also recognized polypeptides in L. tropica, L. donovani and very weakly in L. mexicana promastigotes and in Crithidia lucilliae. The number and size of the polypeptides was different in each species. In addition to the membrane-bound PSA-2 polypeptides we identified water-soluble forms of PSA-2 released in promastigote culture supernatants. Peptide maps of the various L. major PSA-2 membrane polypeptides showed they were different from each other. N-terminal amino acid sequence of the three polypeptides expressed by L. major showed they are similar but distinct, consistent with being members of a polymorphic family. Because of the extensive sequence similarity between the PSA-2 genes it has been difficult to assign protein products to individual genes. As a first step towards solving this problem, we have transfected into L. mexicana a genomic clone of a L. major PSA-2 gene and shown that it produces a M(r) 35,000 polypeptide recognized by monoclonal and polyclonal antibodies to L. major PSA-2.
...
PMID:Characterization of a polymorphic family of integral membrane proteins in promastigotes of different Leishmania species. 783 70

The relative hydrophobicity of ten purified lectins preparations (SBA, LCA, PNA, PSA, STA, WGA, Con A, PHA-P, RCA-I and HPA) was determined using the aqueous two-phase polymeric system Ficoll 400-dextran 70 (13.53% - 11.59%, w/w in H2O, respectively). The linear correlation was found between the relative hydrophobicity of the lectin preparations and their hemagglutinating activity towards native rabbit erythrocytes (r2 = 0.925). Con A specific carbohydrate ligands added to the system decreased the relative hydrophobicity of lectin. Using cross partition, isoelectric points for the lectins were determined.
...
PMID:[Relative hydrophobicity and other properties of lectins in aqueous binary phase polymeric systems]. 839 77

A new method to prepare polyanhydride microspheres capable of near-constant sustained release of low molecular weight, water-soluble molecules is presented. The polyanhydrides used were poly(fatty acid dimer) (PFAD), poly(sebacic acid) (PSA), and their copolymers [P(FAD-SA)]. Acid orange 63 (AO), acid red 8 (AR), and p-nitroaniline, were used as model release molecules. P(FAD-SA) microspheres containing the molecules with or without gelatin were prepared by a modified solvent evaporation method using a double emulsion. The microspheres were spherical with diameters of 50-125 microns and encapsulated more than 85% of the molecule, irrespective of the compound used. Near-zero-order degradation kinetics were observed for 5 days as judged by sebacic acid (SA) release. Microsphere degradation was pH sensitive, being enhanced at high pH, and became more stable in acidic conditions, irrespective of the incorporation of gelatin in the matrix. For the gelatin-free microspheres, a close correlation of SA release and AO release was observed (2% loading), suggesting a release mechanism that was controlled dominantly by degradation. However, the incorporation of gelatin into the microsphere significantly extended the periods of molecule release from P(FAD-SA) microspheres, although the degradation profile of the microspheres themselves was quite similar to that of gelatin-free microspheres. It is possible that an interaction between FAD monomers and gelatin molecules causes continued release, even after the polymer matrix completely degrades (even after complete degradation, FAD monomers remain because of their poor water solubility). Thermal analysis of polyanhydride microspheres at different degradation stages demonstrated that a crystalline structure was formed between gelatin and the FAD monomers produced with microsphere degradation.(ABSTRACT TRUNCATED AT 250 WORDS)
...
PMID:Polyanhydride microspheres that display near-constant release of water-soluble model drug compounds. 846 12

A method to provide near-constant sustained release of high molecular weight, water-soluble proteins from polyanhydride microspheres is described. The polyanhydrides used were poly(fatty acid dimer) (PFAD), poly(sebacic acid) (PSA), and their copolymers [P(FAD-SA)]. P(FAD-SA) microspheres containing proteins of different molecular sizes--lysozyme, trypsin, heparinase, ovalbumin, albumin, and immunoglobulin--were prepared by a solvent evaporation method using a double emulsion. The microspheres containing proteins were spherical, with diameters of 50-125 microns, and encapsulated more than 80% of the protein, irrespective of the protein used. Enzymatic activity studies showed that encapsulation of enzymes inside polyanhydride microspheres can protect them from activity loss. When not placed inside polyanhydride microspheres, trypsin lost 80% of its activity in solution at 37 degrees C at pH 7.4 in 12 hr, whereas inside the polyanhydride microspheres the activity loss was less than 10% under these conditions. About 47% of the enzymatic activity of heparinase encapsulated in the microspheres was lost at 37 degrees C in 24 hr, while in solution it lost over 90% of its activity. The protein-loaded microspheres displayed near-zero-order erosion kinetics over 5 days as judged by the release of sebacic acid (SA) from the microspheres. The microspheres degraded to form SA and FAD monomers. All proteins were released at a near-constant rate without any large initial burst, irrespective of polymer molecular weight and protein loading. The period of protein release was longer than that of SA and continued protein release was observed even after the microsphere matrix had completely degraded. Differential scanning calorimetric studies demonstrated an interaction between protein and the FAD monomers produced with microsphere degradation. It is likely that the protein interaction with FAD monomers permits formation of water-insoluble protein aggregates which slowly dissolve and diffuse out of the matrix, leading to delayed protein release. For trypsin-loaded microspheres, trypsin lost 40% of its activity during microsphere preparation. Activity studies demonstrated that the sonication process was primarily responsible for activity loss. A reduction in the period of ultrasound exposure decreased the loss of protein activity to around 20%.
...
PMID:Controlled delivery systems for proteins using polyanhydride microspheres. 848 30

The purpose of the study has been to observe the influence of an increased dietary sodium intake over cerebral excitability in rats. Research was conducted on two lots of animals: the first lot (PSA) was maintained under the influence of an increased intake of sodium given in the form of physiologic solution, instead of water. That regimen was started during gestation and continued after birth for another 12-14 months before the rats were sacrified. The second lot was given distilled water (DWA) in an identical manner. In other respects, the diet was similar for both lots We compared the following parameters: a) Electrophysiological (electrocorticogram); b) Hydroelectrolytic balance; c) Sodium concentration capacity of the kidney; d) Mineral-corticoid response; e) Motor and motivational behaviour. The data we obtained point to: 1. A shifting of the ECG frequency spectrum towards higher frequency in rats that consumed NaCl in excess. 2. PSA consume significantly more saline solution than DWA, therefore liquid consumption is also greater. Renal elimination of water, Na and K is significantly greater is PSA compared to DWA. Moreover, DWA conserve sodium while PSA conserve water, the respective values being different in a considerable degree in the two lots. 3. The value of the (urinary Na/urinary K) ratio is double in PSA compared to DWA, pointing to a decrease in mineral-corticoid secretion. 5. The animals that have chronically consumed a hypersaline diet show a significantly greater motor agitation compared to the DWA. When free to choose from among physiological solution, water and glucose solution, PSA show no preference for sodium: this points to the absence of obtained motivation for the saline solution The data support the idea that a chronically increased content of dietary NaCl stimulates cerebral excitability.
...
PMID:Influence of increased sodium intake on cerebral excitability. 889 72

Age-dependent spatial memory impairments have been related to a decline in hippocampal plasticity. Highly polysialylated neuronal cell adhesion molecules (PSA-NCAM) show a strong expression during adulthood within regions associated with neuroplastic events. Furthermore, NCAM molecules have been proposed to mediate neuronal plasticity during learning and memory. The aim of the present study was to examine the effect of ageing on the expression of PSA-NCAM within the hippocampus. To investigate whether age-dependent changes in expression of PSA-NCAM were accentuated in aged rats with learning impairment, animals were in a first step assessed for their cognitive abilities using a Morris water maze. Seven-month-old and 24-month-old-rats were tested for their performance in the Morris water maze. The animals were sacrificed and brain sections were processed for PSA-NCAM immunohistochemistry. Ageing was accompanied by an overall decrease in PSA-NCAM-immunoreactivity (-IR) within the forebrain, presenting a important decrease of the number of PSA-NCAM-IR perikarya within the hippocampus. These results were confirmed by Western blot analysis. No difference in PSA-NCAM immunoreactivity was observed in aged rats with or without spatial learning impairment. It is concluded that although changes in PSA-NCAM accompanied the decrease in cognitive abilities, our data did not evidence a causal relationship between these two parameters.
...
PMID:Decrease in highly polysialylated neuronal cell adhesion molecules and in spatial learning during ageing are not correlated. 902 88

Physiological cervicovaginal acidity can partly inactivate human immunodeficiency virus (HIV). Basic semen components should be able to partially neutralize in vivo cervicovaginal pH. The goals of the study were to evaluate the relationship between cervicovaginal pH and presence of semen components in sexually active African women and to assess whether vaginal douching with water performed just after sexual intercourse could significantly reduce semen components and restore physiological cervicovaginal pH. Cervicovaginal secretion (CVS) from 56 heterosexual African women (19 to 45 years old), living in Bangui, Central African Republic, were evaluated for pH, semen components (prostatic acid phosphatase [PAP] and prostatic specific antigen [PSA]), cellularity, and hemoglobin at inclusion and after vaginal douching with 100 ml of water by using a bock. Before douching, semen components were found in 46 of 56 CVS (82%). The mean vaginal pH was 5.2 (range, 3.6 to 7.7), and concentrations of both PAP and PSA correlated positively and strongly with cervicovaginal pH (P < 0.001). After douching, semen components were found in 35 of 56 CVS (62%) (P = 0.03). Cervicovaginal PAP and PSA levels were significantly decreased (respectively, P < 0.0001 and P < 0.01; PAP, -72%; PSA, -87%), as was the total cell count (-60%; P < 0.0001). Furthermore, in CVS previously positive for both PAP and PSA, the mean vaginal pH was significantly decreased (6.5 versus 5.3, P < 0.01); no genital bleeding was observed. Frequent persistence of semen in CVS from heterosexually active African women leads to a shift from acidity to neutrality that could favor male to female HIV transmission. Vaginal douching provides significant elimination of semen after sexual intercourse; it should be considered for study as a supplementary means for the prevention of heterosexual HIV transmission.
...
PMID:In vivo semen-associated pH neutralization of cervicovaginal secretions. 914 79

Compomers are a new class of materials reportedly having the anticariogenicity and the bonding ability to metals similar to glass ionomers while maintaining the high esthetic qualities of composite resins. The purpose of this study was to determine and evaluate the shear bond strength and fracture pattern of a compomer (Dyract) to stainless steel crowns (SSCs) using different mechanical and chemical retention procedures for possible future development of a chair-side technique of producing esthetic SSCs. Thirty-two Unitek SSCs, divided into four groups, were mounted in autopolymerizing acrylic resin so that the resulting specimen has the crown's flat lingual surface projecting above and parallel to the top surface of the acrylic resin block. Dyract was placed in transparent nylon cylinders (3 x 3 mm) and bonded to SSC's surfaces directly (group 1) or following sandblasting of the SSCs (group 2). In group 3, Dyract was bonded to stainless steel lingual cleats that were previously spot-welded to the SSCs. In group 4, Dyract was bonded to sandblasted SSC's surfaces using Scotchbond Multi-Purpose Plus dental adhesive. Specimens were placed in deionized water for 1 hr at 37 degrees C. Shear bond strength was measured using a universal testing machine. The mean (SD) shear bond strengths in MPa for groups 1-4 respectively were as follows: 2.998 (1.381), 9.518 (2.464), 13.909 (1.653), and 9.372 (3.723). One-way ANOVA and Tukey's multiple range tests revealed a statistically significant difference between the groups (P < 0.00001). While no significant difference was found between groups 2 and 4 in which Dyract-PSA prime/adhesive and Scotchbond Multi-Purpose Plus dental adhesive were used, group 3 had significantly higher shear bond strength than other groups. Stereoscopic and SEM examinations revealed adhesive and mixed bond failures. It is concluded that the bond strength of Dyract to SSCs could be enhanced significantly by applying simple mechanical means of retention that could be available in dental offices.
...
PMID:An in vitro comparison of four surface preparation techniques for veneering a compomer to stainless steel. 920 Jan 99

1 2 3 4 5 6 7 8 9 10 Next >>