ÿþ<HTML><HEAD><TITLE>25º Congresso Brasileiro de Microbiologia </TITLE><link rel=STYLESHEET type=text/css href=css.css></HEAD><BODY aLink=#ff0000 bgColor=#FFFFFF leftMargin=0 link=#000000 text=#000000 topMargin=0 vLink=#000000 marginheight=0 marginwidth=0><table align=center width=700 cellpadding=0 cellspacing=0><tr><td align=left bgcolor=#cccccc valign=top width=550><font face=arial size=2><strong><font face=Verdana, Arial, Helvetica, sans-serif size=3><font size=1>25º Congresso Brasileiro de Microbiologia </font></font></strong><font face=Verdana size=1><b><br></b></font><font face=Verdana, Arial,Helvetica, sans-serif size=1><strong> </strong></font></font></td><td align=right bgcolor=#cccccc valign=top width=150><font face=arial size=2><strong><font face=Verdana, Arial, Helvetica, sans-serif size=1><font  size=1>ResumoID:2138-1</font></em></font></strong></font></td></tr><tr><td colspan=2><br><br><table align=center width=700><tr><td>Área: <b>Micobacteriologa ( Divisão C )</b><p align=justify><strong><P>BIOCHEMICAL AND STRUCTURAL&NBSP;STUDIES OF HISTIDINOL DEHYDROGENASE FROM <EM>MYCOBACTERIUM TUBERCULOSIS</EM></P></strong></p><p align=justify><b><u>José Eduardo Sacconi Nunes </u></b>  (<i>INCT-TB</i>); <b>Rodrigo  Gay Ducati </b>  (<i>INCT-TB</i>); <b>Ardala  Breda </b>  (<i>INCT-TB</i>); <b>Bibiana  Monson de Souza </b>  (<i>INCT-TB</i>); <b>Mario Sergio  Palma </b>  (<i>INCT-TB</i>); <b>Luiz Augusto  Basso </b>  (<i>INCT-TB</i>); <b>Diógenes  Santiago Santos </b>  (<i>INCT-TB</i>)<br><br></p><b><font size=2>Resumo</font></b><p align=justify class=tres><font size=2><P class=MsoNormal style="MARGIN: 0in 0in 0pt; TEXT-INDENT: 35.4pt; TEXT-ALIGN: justify"><SPAN style="mso-ansi-language: EN-US">The aetiological agent of tuberculosis (TB), <EM>Mycobacterium tuberculosis</EM>, was responsible for approximately 1.8 million deaths in the year of 2007. The increasing prevalence of TB, the emergence of multidrug-resistant and extensively drug-resistant strains of the tubercle bacillus, and the devastating effect of co-infection with the human immunodeficiency virus have led to an urgent need for the development of new and more efficient antimycobacterial drugs. The histidine biosynthetic pathway is present in bacteria, archaebacteria, lower eukaryotes and plants, but is absent in mammals. Disruption of the <EM>M. tuberculosis</EM> hisD-encoded L-histidinol dehydrogenase gene by homologous recombination resulted in mutants that were not viable under histidine deprivation. Thus, the gene products of this pathway represent attractive targets for the development of antimycobacterial agents. Although analysis of the complete genome sequence of <EM>M. tuberculosis</EM> predicts that the locus-tag Rv1599 (hisD) codes for a probable histidinol dehydrogenase (MtHisD) enzyme, experimental evidence was lacking. The <EM>M. tuberculosis</EM> hisD gene was PCR amplified, cloned, sequenced, and the recombinant protein was overexpressed and purified. MtHisD enzyme activity measurements of soluble protein cellular extracts of recombinant protein demonstrated a 612-fold increase in specific activity as compared to control cell extracts. Furthermore, steady-state velocity of recombinant MtHisD showed a linear dependence on cell extract volume added to the reaction mixture. Apparent steady-state kinetic constants were determined with the pure enzyme. The results reported here validate hisD as the structural gene that codes for histidinol dehydrogenase in <EM>M. tuberculosis</EM>, and along with its proposed three-dimensional model, provide material for structural and mechanistic studies aiming at the rational design of new anti-TB agents.<?xml:namespace prefix = o ns = "urn:schemas-microsoft-com:office:office" /><o:p></o:p></SPAN></P></font></p><br><b>Palavras-chave: </b>&nbsp;Enzyme Kinetics, Histidinol Dehydrogenase, Homology Modeling, Mycobacterium tuberculosis</td></tr></table></tr></td></table></body></html>