Estudos das enzimas adenosina kinase e hipoxantina-guanina fosforibosiltransferase de Schistosoma mansoni

Romanello, Larissa

Estudos das enzimas adenosina kinase e hipoxantina-guanina fosforibosiltransferase de Schistosoma mansoni

Detalhes bibliográficos
Ano de defesa:	2011
Autor(a) principal:	Romanello, Larissa
Orientador(a):	Garratt, Richard Charles
Banca de defesa:	Não Informado pela instituição
Tipo de documento:	Dissertação
Tipo de acesso:	Acesso aberto
Idioma:	por
Instituição de defesa:	Universidade Federal de São Carlos
Programa de Pós-Graduação:	Programa de Pós-Graduação em Biotecnologia - PPGBiotec
Departamento:	Não Informado pela instituição
País:	BR
Palavras-chave em Português:	Enzimas Schistosoma mansoni Cristalografia de proteínas Adenosina kinase Hipoxantina-guanina fosforibosiltransferase
Área do conhecimento CNPq:	CIENCIAS BIOLOGICAS
Link de acesso:	https://repositorio.ufscar.br/handle/ufscar/6981
Resumo:	Schistosoma mansoni is the parasite responsible for schistosomiasis mansonica, a disease that affects about 207 million people worldwide, and does not have the purine de novo sinthetic pathway, depending entirely on the purine salvage pathway to supply its demands on purines. Adenosine kinase (AK) and Hypoxanthine-guanine phosphoribosyltransferase (HGPRT) are important enzymes of the purine salvage, the AK directly phosphorylates adenosine into adenosine monophosphate (AMP) and HGPRT is responsible for the reversible phosphorybosylation of hypoxanthine or guanine into IMP or GMP. The purine salvage pathway has been reported as a potential target for developing new drugs against schistosomiasis. The nucleotide coding region of the isoform 2 of AK enzyme was amplified and cloned into pGEM vector and pET28a, the recombinant protein was expressed in E.coli BL21 (DE3), purified in a his-tag nickel-affinity resin and AMP-agarose resin, tested for its activity and crystallized. Two data sets were obtained by X-ray diffraction: a ternary complex of AK2-AMP-adenosine in the MX2 light line of the Synchrotron Light National Laboratory and a binary complex AK2-tubercidin in the rotatory anode X-ray source of the Institute of Physics at Sao Carlos - USP, both at 2.3A of resolution. The nucleotide coding region of the enzyme HGPRT was also amplified, cloned into pGEM and pET28a, which heterologous expression was done in E.coli BL21 (DE3) cells at 18°C and purified on a cobalt his-tag affinitiy resin.

Estudos das enzimas adenosina kinase e hipoxantina-guanina fosforibosiltransferase de Schistosoma mansoni

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