Wahrnehmung von Biotinmangel durch Saccharomyces cerevisiae

Stüer, Heike

January 2009

Regensburg, Univ., Diss., 2009.

Biotin-dependent modifications of histones

Camporeale, Gabriela.

January 1900

Thesis (Ph.D.)--University of Nebraska-Lincoln, 2006. / Title from title screen (sites viewed on August 10, 2006). PDF text of dissertation: 98 p. : ill. ; 1.16Mb. UMI publication number: AAT 3208087. Includes bibliographical references. Also available in microfilm, microfiche and paper format.

The Effect of Avidin Injected Intraperitoneally on the Course of Leukemia in the Mouse / The Effect of Avidin Injected Peritoneally on the Course of Leukemia in the Mouse

Jones, George Adams, III

01 1900

The current work was undertaken to test the ability of avidin to affect the course of leukemia when administered intraperitoneally.

leukemia

biotin

Avidin.

Leukemia -- Treatment.

Transition metal catalyzed alkylation and synthesis of biotin derivatives

Shen, Di

January 2014

<b>Transition Metal Catalyzed Alkylation</b> We have reported methodology for the use of methanol as an alkylation reagent using catalytic rhodium or iridium species for the formation of branched products from methyl ketones. The synthetic utility of the dialkylated products was enhanced by performing a regioselective Baeyer-Villiger oxidation which allowed access to ester products. A range of different phosphine ligands were screened, and sterically hindered and electron rich phosphine ligands were found to favour the formation of enone and methoxy adducts under an O2 atmosphere. This interrupted hydrogen borrowing reaction enabled the in situ addition of a nucleophile to give more complex products. A range of tetrasubsitituted pyridines were then synthesized from 1, 5-dicarbonyl compounds formed in the methylenation/conjugate addition sequence. Finally, deuteration experiments suggest that the reaction proceeds via a monohydride mechanism, and the possibilities for the beneficial effect of O2 were discussed. <b>Synthesis of biotin derivatives</b> The streptavidin-biotin system was chosen for the studies of protein/ligand interactions at molecular level. A series of modified biotin ligands were designed and synthesized to introduce repulsive interations with streptavidin. The protein/ligand complexes were analyzed at high resolution by X-ray crystallography.

547

Photo-switching of protein activities by conjugation of photo-responsive polymers to proteins /

Shimoboji, Tsuyoshi.

January 2001

Thesis (Ph. D.)--University of Washington, 2001. / Vita. Includes bibliographical references (leaves 165-172).

Biotin protein ligase from Saccharomyces cerevisiae /

Polyak, Steven William.

January 2000

Thesis (Ph.D.)--University of Adelaide, Dept. of Biochemistry, 2000? / Bibliography: leaves 130-159.

Der Effekt von Sirolimus auf die reaktive Zellproliferation und Apoptose in einem humanen ex vivo Restenose-Modell

Zellmann, Svenja,

January 2007

Ulm, Univ., Diss., 2007.

Molecular recognition in the streptavidin-biotin system /

Chu, Vano.

January 1998

Thesis (Ph. D.)--University of Washington, 1998. / Vita. Includes bibliographical references (leaves [66]-73).

Effect of biotin supplementation on the metabolism of lactating dairy cows

Ferreira, Gonzalo,

January 2006

Thesis (Ph. D.)--Ohio State University, 2006. / Title from first page of PDF file. Includes bibliographical references (p. 101-118).

Studies on biotin as a coenzyme of propionyl carboxylase

Kosow, David Phillip

January 1962

A soluble enzyme system has been isolated from biotin-deficient rat liver acetone powder which catalyzes the synthesis of propionyl holocarboxylase from d-biotin and its apocarboxylase, in the presence of ATP and Mg++ ions. The enzyme system has been partially purified by (NH₄)₂SO₄ precipitation and resolved into two obligatory components by alumina C y gel fractionation. The gel supernatant fraction has been further purified by DEAE cellulose ion-exchange chromatography. Since the active component in the gel supernatant fraction and the endogenous propionyl holocarboxylase have the same elution pattern when chromatographed on DEAE cellulose, it appears likely that the gel supernatant contains the propionyl apocarboxylase. The gel eluate most likely contains an enzyme which catalyzes the covalent bonding or d-biotin to propionyl apocarboxylase and other proteins. In order to measure the activity of the propionyl holocarboxylase synthesizing system, two assay procedures were used. One assay procedure employed the incorporation of biotin-1-c¹⁴ into protein as a measure or the activity of the enzyme system. The other assay was based upon the biotin and ATP dependent increase of propionyl carboxylase activity catalyzed by the enzyme system. Both procedures gave similar results. Propionyl holocarboxylase formation was found to be ATP specific since neither CTP, OTP, ITP, nor UTP could replace ATP. In addition, a mixture or all five nucleoside triphosphates was no more effective than ATP alone. Versene inhibited the reaction and MgCl₂ was able to reverse this inhibition, indicating a Mg++ ion requirement. The ability of various biotin derivatives to replace d-biotin in propionyl holocarboxylase formation was investigated. It was round that if either the valeric acid side chain is altered. as in homo- or nor-biotin, of if the sulfur atom is removed or substituted, as in desthiobiotin or oxybiotin, holocarboxylase formation did not occur. Similarly, neither of these derivatives inhibited the bonding of c¹⁴-biotin to protein. Biocytin has been eliminated as an intermediate in propionyl holocarboxylase formation. Hydroxylamine does not inhibit the reaction. nor is CoA required. These data would appear to eliminate the involvement of free carboxyl activated biotinyl intermediates in the formation of the holocarboxylase from its apocarboxylase and biotin. Although the evidence suggests a concerted mechanism for the reaction, mechanisms involving enzyme bound intermediates are not completely eliminated by these data. In order to determine the nature of the attachment of biotin to propionyl carboxylase, c¹⁴-biotin labeled propionyl carboxylase was prepared. The labeled carboxylase was enzymatically hydrolyzed and chromatographed on Whatman 3MM paper. The biocytin peak contained nearly 100% of the radioactivity recovered. This peak was eluted and rechromatographed by ion-exchange chromatography. The only radioactive component obtained by this procedure was biocytin. The data presented indicate that the propionyl holocarboxylase synthesizing system catalyzes the ATP dependent covalent bonding of d-biotin to the lysyl-(-amino groups or propionyl apocarboxylase. / Ph. D.

LD5655.V856 1962.K676

Biotin

Decarboxylases