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Non-Phosphorylating And Phosphorylating Oxidoreductase Glyceraldehyde-3-Phosphate Dehydrogenase As Part Of A Structure-Based Design In Glycolysis As The Glycolytic Protein G3PD.

Glyceraldehyde-3-phosphate dehydrogenase (EC 1.2.1.12) GAPDH1/G3PD, is located in band 12p13.31; related to both glycolysis2 and gluconeogenesis-pathways. G3PD catalyzes reversible oxidative phosphorylation of inorganic phosphate and nicotinamide3 adenine dinucleotide (NAD)4 converting in glycolysis the glycolytic protein GAPDH5 in which adenosine-triphosphate (ATP)6 is generated when phosphoglycerate kinase (PGK)7 is produced in the GAPDH8-catalyzed reaction. These intermediate metabolites (aldolase9, triose-phosphate10-isomerase (TPI)11) catalyze the Glycolysis reactions, in the sequence of the ten enzyme-catalyzed Embden12Meyerhof13 reactions in the metabolic pathway. Converting phosphoglycerate mutase 1 (PGM)14 catalyzing the internal steps by 2,3-BPG15 phosphatase to form by converting D-glyceraldehyde 3-phosphate (G3P)16 into 1,3-bisphosphoglycerate (1,3-BPG)17 from its role as 3-Phosphoglyceric acid (3PG) in glycolysis as the glycolytic protein GAPDH18 that catalyzes the first step (G3P19 into 1,3-BPG) of the pathway. Plant20 cells contain several reactions of photosynthesis21 participating in glycolysis and the Calvin-Benson22 cycle signaling pathways in plants (cytosolic-GAPC23 (Arabidopsis thaliana)24 functions in plant25 cells.) its final byproduct is also another Glyceraldehyde-3-P. GAPDH is a band 326 protein that associates with the cytoplasmic27 face of human erythrocyte28 (RBC)29 membranes. The cytoplasmic GAPDH exists primarily as a tetrameric30 isoform, 4 identical 37 kDa31 subunits. By subcellular translocation GAPDH32 participates in nuclear events [In nuclear membrane the vesicular33 tubular cluster fractions34 (VTCs)35 – anterograde transport or retrograde36 membrane transport complexes37 between the intermediates, these are the Golgi38 complex and the endoplasmic reticulum (ER)39, in the nucleus a function is lost in disease that exploits this process.], this a change to a non-cytosolic40 localization due to the signal transduction pathways (considering Lm41GAPG L.42 mexicana43-like functions.) involved in s-nitrosylase44 activity that mediates, governed by the equilibrium between four cysteine residues (nitrosylation45 and denitrosylation reactions)46, inhibition of GAPDH nuclear translocation, as a basis47 for its multifunctional48 activities relating to the extraglycolytic functions of GAPDH. Nuclear GAPDH49 promotes glucose metabolism to sustain50 cellular ATP51 levels, or potentially by inhibiting targets52 of p30053/CBP such as p5354 dependent phosphorylation. Nitric oxide synthase or neuronal NOS ( involved in cellular and human intracellular55 nuclei events56, in addition to the cytoplasm) could generate nitric oxide57 (NO). GAPDH has four cysteine58 residues which are associated with S-nitrosylation59-yielding NOS60-GAPDH which “recruited” its glycolysis subunit61 from the three63 molecular axes translocation roles (S-thiolation64, S-nitrosylation or aggregated65 enzymes (Cys-15266 and nearby 15667 converted into a ‘cross-linked68 soluble’ states)), and (SNO69-GAPDH) nitrosylated S-nitrosoglutathione70 (GSNO)71 the active site cysteine residue in GAPDH at its Cys 15072 residue that binds to Siah1 (seven in absentia homolog 1) acquisition and the translocation of GAPDH into the nucleus, and denitrosylation using a combination of approaches, including G3P73 . And NADPH may play a role in (VTC) vesicle74 function. The complex would function in the apoptosis cascade75 by its molecules translocation, this may76 depend on lysine 22777 in the human GAPDH78Siah79 interaction to another intracellular position80 induced by apoptotic81 stimuli, augments p30082/CREB binding protein (CBP)-associated83 acetylation of nuclear proteins. ‘Engineering the cofactor (GAPDH-(Lys) K160R84-K227A) availability prevents85 activation of p300/CBP that interferes with GAPDH-Siah1 binding86-prevents the ternary (GAPDH-Siah1) complex associations translocation; that CGP-346687 can reduce independently with both cofactors88. Dysregulation of protein S-nitrosylation (S-nitrosocysteine89247) by lipopolysaccharide (LPS) is associated with pathological90 conditions which contributes to disease phenotype, where GAPDH protects ribosomal protein RP91L13a92 from degradation, L13a93 and GAPDH94 forms a functional GAIT95 complex. One of the functions of GAPDH proteins role in glycolysis96 in relation to DNA97 synthesis is nuclear accumulation associated by the NAD98(+)-dependent s-nitrosylation99 and denitrosylation01 reactions both of these isforms are distinct02 parallel to the uracil DNA glycosylase (UDG)03 gene in mitochondria04 and in the nucleus is N-terminally processed is the 37-kDa subunit05 of the (GAPDH)06 glyceraldehyde-3-phosphate dehydrogenase protein. This enzyme is an example of moonlighting protein which is validated and replaced07 by alternative reference genes that link (in their nuclear forms) on the multifunctional08 properties of the enzyme GAPDH09 known as a key enzyme in glycolysis that contributes to a number of diverse cellular functions unrelated00 to glycolysis001 depending upon its subcellular location. GAPDH is a key enzyme in glycolysis the most commonly used expression is as a housekeeping002 gene.

Cytotoxic stimuli [1a.] or Programmed cell death, via nitric oxide generation, lead to the binding of GAPDH from its usual tetrameric form to a dimeric form, to the protein Siah1 [1.] intracellular G-3-P [2.] substrate [3.] protects GAPDH from S-nitrosylation [4.]. The GAPDH-Siah interaction depends on lysine 227 [5.], in human GAPDH that interacts with a large groove [6.] of the Siah1 dimer, that connects the GAPDH dimer to PGK in the cytoplasm. figure7The S-nitrosylation [7.,8.] abolishes catalytic activity and confers upon GAPDH the ability to bind to Siah [9.]. (GAPDH) is physiologically nitrosylated at its Cys 150 residue. GAPDH (SNO-GAPDH) [10.] binds to Siah1 [11.] by forming a protein complex. In the nucleus [12.] GAPDH is acetylated at Lys 160 [13.] and binds to the protein acetyltransferase p300/CBP. Under these conditions siah-1 formed a complex with GAPDH (PDB:4O63) and localized in the nucleus of Müller cells [14.]. GAPDH mutants [15.] that cannot bind Siah1 prevents translocation [16.] to the nucleus to elicit neurotoxicity [17.] and cell apoptosis.

[1a.] 16492755, 8769851003 [1.]16391220, [2.]19542219, 22534308, 3350006004, 19937139, [3.]22847419, [4.]15951807, [5.]20601085, [6.]16510976, 20392205005, [7.,8.]22817468006, 16505364007, [9.]16633896, [10.]16574384, [11.]20972425, [12.]19607794, [13.]18552833, [14.]19940145, [15.]23027902008, [16.]24362262, [17.]16492755.

Analysis of CGP-3466 Docking (NAD) to Human Placental GAPDH which decreases the synthesis of pro-apoptotic proteins is N-terminally PMID:10677844, processed to which a Rossmann NAD(P) binding fold as seen in figure 1 is a C-terminal domain as seen on this page, PMID:10617673, 26022259, 16510976 …The structure is also used to build a model of the complex between GAPDH and the E3 ubiquitin ligase Siah1. (Purple Ribbon-1U8F_Q Figure 1.)

In the GAPDH-catalyzed reaction these intermediate metabolites (aldolase, triose-phosphate-isomerase Glycolysis and Glyconeogenesis (TPI)) catalyze the Glycolysis reactions, in the sequence of the ten enzyme-catalyzed Embden-Meyerhof reactions in the  metabolic pathway. Converting phosphoglycerate mutase 1 (PGM) catalyzing the internal steps by 2,3-BPG phosphatase to form by converting D-glyceraldehyde 3-phosphate g3p(G3P) into 1,3-bisphosphoglycerate (1,3-BPG) from its role as 3-Phosphoglyceric acid (3PG) in glycolysis as the glycolytic protein GAPDH that catalyzes the first step (G3P into 1,3-BPG) of the pathway.

GAPDH homotetramer was studied as represented an assembly of repeating spherical units that harbored a distinct birefringent crystal structure to the optic axis for the p polarization, also (r axis) discernible via transmission electron microscopy. of the relative amount of soluble monomeric GAPDH to G3P in the binding pocket of the NAD(+)-binding site residue located at the active site linked to GAPDH in Figures 5 and 6. PMID:10407144009, 25086035.

g3pAnother model building studie indicates that a structure obtained where glyceraldehyde 3-phosphate PDB:3CMC_Q binds in the P(s) pocket of the natural substrate G3P phosphorylating GAPDH (PDB:1U8F_Q) at the catalytic cysteine residue site. To define the conditions suitable for affinity for the cosubstrate, the isolation and accumulation of the intermediate metabolites per G3P monomer found in Figure 8 of the equivalent Glc-3-P structure in the binding pocket of the NAD(+)-binding site residue located at the active site linked to GAPDH. PMID:19542219, 22534308

Correctly known binding sites on ((GAPD/NAD)) structures, polar spheres of the binding catalytic pocket that corresponds to G3P (glyceraldehyde 3-phosphate) aligned to the holographical structure nonbounded spheres (salmon color), these apoenzymes together with the cofactor(s) Cys 151, 152 which corresponds as below the Ps pocket of G3P, on the Green ribbon required for cofactor activity. Together with eliminated crystallographic waters and other possible spheres, these are at least one atom of a amino acid residue in contact with at least one alpha sphere of one binding pocket on the holo protein NAD structure 1U8F_Q needed to align holo and apo structures included in this data set with G3P (PDB:3CMC_Q) was tested only on holo structure (NAD), obtained via Pea Green spheres aligned to 1U8F_Q ribbons/ligand structure which provide structural recognition insights into the biological 1U8F-Q assembly this includes 29 asymmetric units of its dimeric form, along the tetrameric 1U8F biological forms axis. PMID:9461340010

(Figure 8.) These are the results without the liquid chromatography coupled mass spectrometer, that are known 3D products by two-dimensional sequence analyses with the STRAP alignment tools data sets and which may have any effect on the functions of further analysis involved in more ordered results than this study attempts to show, of the analysis that may be included are identified separated into multiple gradients here in these paired graphs. Therefore in the present work to uncover the exact coincidence of 1U8F_R and 4I7D_C, the 3D coordinates of GAPDH (PDB:1U8F_Q) to the protein Siah1 4I7D were not presenting when subjected to STRAP  alignment this apparent discrepancy (Figure 1.) was partially resolved by a (Figure 7) rendering from a more reactive native GAPDH_R homotetramer model.

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