Silicon Investor (SI) -- The First Internet Community

STOCKTALK

We've detected that you're using an ad content blocking browser plug-in or feature. Ads provide a critical source of revenue to the continued operation of Silicon Investor. We ask that you disable ad blocking while on Silicon Investor in the best interests of our community. If you are not using an ad blocker but are still receiving this message, make sure your browser's tracking protection is set to the 'standard' level.

Biotech / Medical : Millennium Pharmaceuticals, Inc. (MLNM) -- Ignore unavailable to you. Want to Upgrade?

To: tuck who wrote (2316)	2/14/2006 10:43:34 AM
From: tuck	Read Replies (1) \| Respond to of 3044

[MLN-273/proteasome inhibition versus tuberculosis] >>Mol Microbiol. 2006 Mar;59(5):1417-28. Structure of the Mycobacterium tuberculosis proteasome and mechanism of inhibition by a peptidyl boronate. Hu G, Lin G, Wang M, Dick L, Xu RM, Nathan C, Li H. Biology Department, Brookhaven National Laboratory, 50 Bell Avenue, Upton, NY 11973, USA. Mycobacterium tuberculosis (Mtb) has the remarkable ability to resist killing by human macrophages. The 750 kDa proteasome, not available in most eubacteria except Actinomycetes, appears to contribute to Mtb's resistance. The crystal structure of the Mtb proteasome at 3.0 A resolution reveals a substrate-binding pocket with composite features of the distinct beta1, beta2 and beta5 substrate binding sites of eukaryotic proteasomes, accounting for the broad specificity of the Mtb proteasome towards oligopeptides described in the companion article [Lin et al. (2006), Mol Microbiol doi:10.1111/j.1365-2958.2005.05035.x]. The substrate entrance at the end of the cylindrical proteasome appears open in the crystal structure due to partial disorder of the alpha-subunit N-terminal residues. However, cryo-electron microscopy of the core particle reveals a closed end, compatible with the density observed in negative-staining electron microscopy that depended on the presence of the N-terminal octapetides of the alpha-subunits in the companion article, suggesting that the Mtb proteasome has a gated structure. We determine for the first time the proteasomal inhibition mechanism of the dipeptidyl boronate N-(4-morpholine)carbonyl-beta-(1-naphthyl)-l-alanine-l-leucine boronic acid (MLN-273), an analogue of the antimyeloma drug bortezomib. The structure improves prospects for designing Mtb-specific proteasomal inhibitors as a novel approach to chemotherapy of tuberculosis.<< Cheers, Tuck

To: tuck who wrote (2316)	9/11/2007 11:45:08 AM
From: tuck	Respond to of 3044

[Chronic Proteasome Inhibition Contributes to Coronary Atherosclerosis] >>Circ Res. 2007 Sep 6; [Epub ahead of print] Chronic Proteasome Inhibition Contributes to Coronary Atherosclerosis. Herrmann J, Saguner AM, Versari D, Peterson TE, Chade A, Olson M, Lerman LO, Lerman A. Divisions of Cardiovascular Diseases and Nephrology and Hypertension, Department of Internal Medicine, Mayo Clinic and College of Medicine, Rochester, Minn. The proteasome is responsible for the degradation of oxidized proteins, and proteasome inhibition has been shown to generate oxidative stress in vitro. Atherosclerosis is thought to be initiated as a consequence of increased endogenous oxidative stress. The current study was designed to assess whether chronic proteasome inhibition is associated with early coronary atherosclerosis. Female pigs, 3 months of age, were randomized to a normal (N) or high-cholesterol (HC) diet (2% cholesterol, 15% lard) without or with twice weekly subcutaneous injections of the proteasome inhibitor (PSI) MLN-273 (0.08 mg/kg, N+PSI and HC+PSI) for a period of 12 weeks (n=5 per group). Coronary vasorelaxation to bradykinin (10(-10.5) to 10-(6.5) mol/L) and sodium nitroprusside (10(-9) to 10(-5) mol/L) was assessed by in vitro organ chamber experiments, intima-media ratio by morphometric analysis of Elastica-van Gieson-stained slides, and intima superoxide production by dihydroethidium fluorescence. Vasorelaxation to 10(-6.5) mol/L bradykinin was reduced in HC compared with N (69+/-7 versus 90+/-2%, P<0.05) and further reduced in N+PSI and HC+PSI (57+/-6 and 48+/-13%, P<0.05 versus N and HC for each). Compared with N (0.03+/-0.01), intima-media ratio was higher in N+PSI (0.09+/-0.04, P<0.01) and HC+PSI (0.15+/-0.06, P<0.05). Compared with N (0.6+/-0.9% of intima area), dihydroethidium fluorescence was higher in HC, N+PSI, and HC+PSI (8.9+/-1.6, 6.0+/-3.5, and 7.2+/-3.9% of intima area, P<0.05 for all). Thus, chronic proteasome inhibition is associated with increased coronary artery oxidative stress and early atherosclerosis. These findings support the significance of the proteasome and related protein quality control for vascular biology and pathology.<< Cheers, Tuck