UMLS:C0027960 - FACTA Search

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Query: UMLS:C0027960 (mole)
21,279 document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)

A most significant decrease of prealbumin and retinol-binding protein was observed in the serum during an absolute alimentary abstinence for five days, whereas the immunoglobulins IgG, IgA and IgM were not influenced. The decrease in the concentration of prealbumin and retinol-binding protein was significantly diminished through a minimum diet of 15 g essential aminoacids and 60 g carbohydrates. Both proteins form a complex in a mole ratio of 1:1. Based on the four to five times higher prealbumin concentration, we recommend this parameter for the routine observation of protein metabolism during weight reduction.
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PMID:[Blood proteins during short-term fasting and during supply of essential amino acids]. 56 76

Vitamin A-transporting protein in chicken plasma was purified by column chromatography on DEAE-Sephadex and Sephadex G-100; the protein formed a complex of retinol-binding protein (RBP) with prealbumin (PA). The molecular weight of the 1:1 molar complex was estimated to be 76,000 by gel filtration, and the sedimentation coefficient (S20,W) was found to be 5.2 S. RBP and PA were dissociated from the purified complex by means of CM-Sephadex column chromatography. Purified RBP contained 1 mole of vitamin A bound per mole of RBP. The molecular weight of RBP was determined to be 20,000 by gel filtration on Sephadex G-75, 19,000 by SDS-disc gel electrophoresis, and 20,500 by sedimentation equilibrium analysis. The S20,W was calculated to be 2.0 S. The molecular weight of PA was determined to be 56,000 by gel filtration, 52,000 by sedimentation equilibrium analysis, and 13,000 by SDS-disc gel electrophoresis. The S20,W was calculated to be 3.9 S. From these findings it was concluded that PA consists of four subunits, each with a molecular weight of approximately 13,000. Peptide mapping experiments suggested that the subunits were identical. No carbohydrates were detected in either RBP or PA. Chicken RBP and PA were immunologically distinct from those of human and rat. It is well established that vitamin A is transported bound to a specific plasma protein, retinol-binding protein (RBP), in both man (1,2) and rat (3). Purified human and rat plasma RBP have a single binding site for one molecule of retinol, alpha mobility on disc gel electrophoresis, and a molecular weight of approximately 20,000. In both species, RBP forms a tight complex with plasma prealbumin (PA) and normally circulates as a 1:1 molar protein-protein complex with PA (1-5). Despite these similarities, no immunological cross-reactivity between human and rat RBP has been observed (3,6). The present study was undertaken to explore whether or not a similar transport system for vitamin A exists in the chicken, a nonmammalian vertebrate. During the course of this study, Mokady and Tal (7) reported the isolation of RBP from chicken plasma and some physicochemical properties, e.g., a molecular weight of about 19,000. On the other hand, Muto, Smith, and Goodman (6) had already observed that the molecular weight of vitamin A-containing protein in fresh chicken plasma is approximately 60,000-80,000, as determined by gel filtration. However, no convincing information is available regarding an entire system of vitamin A transport in chicken plasma. We now describe procedures for the isolation of the RBA-PA complex of chicken plasma and the dissociation into the component proteins, RBP and PA. We also describe in detail the physicochemical properties of the individual proteins. It is also clearly demonstrated that chicken RBP and PA are immunologically distinct and different from the respective proteins in man and rat. Moreover, purified chicken PA appears to be a tetramer of four identical subunits and is thus similar to human and rat PA.
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PMID:Vitamin A transport in chicken plasma: isolation and characterization of retinol-binding protein (RBP), prealbumin (PA), and RBP--PA complex. 80

Thyroxine-binding alpha globulin (TBG) in human serum was isolated from Cohn fractions IV-5,6 and IV-4 by (1) chromatography on carboxymethyl (CM) cellulose, (2) gel filtration on Sephadex G-200, (3) chromatography on diethylaminoethyl-Sephadex, (4) a novel procedure of "double-gel" electrophoresis, and (5) preparative polyacrylamide gel electrophoresis. The protein was homogeneous by analytical disc gel electrophoresis, immunoelectrophoresis, and ultracentrifugal analyses (sedimentation velocity and sedimentation equilibrium), and after addition of thyroxine-(125)I showed a constant specific radioactivity on polyacrylamide electrophoresis. The sedimentation and diffusion coefficients were s(20, w), 3.0 x 10(-13) sec, and D(20, w), 8.05 x 10(-7) cm(2).sec(-1), and the molecular weight obtained by sedimentation equilibrium was 36,500. Gel filtration studies on Sephadex G-200 demonstrated that the protein had the same elution volume as that of native TBG in serum, apparently excluding the possibility of a subunit of the native protein. Chemical composition was ascertained by amino acid and carbohydrate analyses. The maximal thyroxine (T4)-binding capacity measured by reverse flow paper electrophoresis was 15,000 mug per g of protein, representing more than 2100 times that of the starting material, or about 5000 times that of whole serum. Based on the molecular weight obtained, the TBG preparation could bind 0.7 mole T4 per mole of protein, suggesting a single binding site. The association constant for T4 was estimated to be of the order of 10(10) by competitive binding studies employing TBG and T4-binding prealbumin (TBPA).
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PMID:Preparation and properties of thyroxine-binding alpha globulin (TBG). 410 64

A euthyroid adult female (LC) was found to have persistently raised concentrations of total T4 (159 nmol/l) and rT3 (500 pmol/l) in her serum in association with a normal T3 (2.1 nmol/l). Serum concentrations of all three T4-binding proteins were within normal limits. A variant prealbumin with an increased affinity for T4 was found to be responsible for the raised serum level of T4. Unlike normal prealbumin, the variant also bound appreciable amounts of rT3. The affinity constant for T4 binding to prealbumin LC was 5.5 X 10(8) l/mole which is sevenfold higher than that obtained for normal prealbumin (8.5 X 10(7) l/mole). The affinity constant for the binding of rT3 to prealbumin LC was 2.0 X 10(6) l/mole while that for the normal protein was unmeasurable by our method. The T4-binding capacity of prealbumin LC in serum was within the normal range indicating that there is no new additional T4-binding site on the protein. Prealbumin LC has the same molecular size as the normal protein, hence it is likely that the tetrameric structure has been preserved. The electrophoretic mobility of prealbumin LC was normal indicating no alteration in charge. It is postulated that the increased affinity for T4 (and presumably for rT3) results from a hydrophobic amino-acid substitution in the prealbumin monomer.
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PMID:A prealbumin variant with an increased affinity for T4 and reverse-T3. 643 33

A 900- to 1100-bp fragment encompassing intron 1 of the nuclear transthyretin (prealbumin) gene was examined in 12 taxa of Old World hystricognath rodents of the families Bathyergidae, Petromuridae, Thryonomyidae, and Hystricidae. Within the Bathyergidae, Heterocephalus glaber (naked mole-rat) was basal, and the other East African species, Heliophobius argenteocinereus (silvery mole-rat), was sister to a southern African clade containing Bathyergus, Cryptomys, and Georychus (dune, common, and cape mole-rats). These results are congruent with studies using mitochondrial 12S rRNA gene sequences. A combined analysis of transthyretin and 12S rRNA data resulted in a well-supported topology with better resolution than either gene analyzed separately. These data support the findings by M. W. Allard and R. L. Honeycutt (1992, Mol. Biol. Evol. 9: 27-40) and R. L. Honeycutt (1992, Am. Sci. 80: 43-53) that complex social systems evolved independently at least twice, in the common and naked mole-rats.
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PMID:Evidence from intron 1 of the nuclear transthyretin (Prealbumin) gene for the phylogeny of African mole-rats (Bathyergidae). 1099 98

We report the production of a new monoclonal antibody, PNL2, directed against a fixative resistant melanocyte antigen. The analysis of PNL2 immunostaining on a broad range of normal or malignant human tissues and on various melanocytic lesions revealed its high specificity. PNL2 gave a strong cytoplasmic staining of skin and oral mucosae melanocytes, and staining of granulocytes when used at high concentration. PNL2 stained all intra-epidermal nevi irrespective of their histologic type, but common intradermal nevi and the dermal component of compound nevi were largely non-reactive as only scattered nevus cells in the papillary dermis were labeled. PNL2 labeled more than 70% of the neoplastic cells in all primary melanomas irrespective of their histologic type. However, PNL2 did not label desmoplastic melanomas. All metastatic melanomas were also stained but the percentage of labeled cells was occasionally lower than the primary tumor. PNL2, as anti-Melan A and HMB-45 antibodies, stained most of the clear cell sarcoma cells, and a few cells in angiomyolipomas and lymphangioleiomyomatosis. None of the other non-melanocytic lesions tested were labeled. Proteomic approaches showed that the immunoaffinity purified PNL2-binding complexes isolated from melanoma cell lines comprise at least TAP1, Clathrin 17 and prealbumin proteins, but not the gp100 recognized by HMB-45. In conclusion, this new monoclonal antibody, PNL2, is directed against a new fixative resistant melanocyte associated antigen. This antigen is chemically resistant and thus allows immunostaining after melanin bleaching or decalcification. We also demonstrate that it is different from Melan A and from gp100, even if PNL2 and HMB-45 staining patterns are sometimes similar.
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PMID:PNL2, a new monoclonal antibody directed against a fixative-resistant melanocyte antigen. 1274 55