Structuro-functional characteristics of aldolase from rabbit muscles in diabetes

The structural peculiarities of rabbit muscle aldolase accompanying enhancement of the aldolase activity in diabetes are described from the data of tryptophan phosphorescence at the room temperature and fluorescence polarization. It is shown that the pathology-concomitant conformational changes occur in both the hydrophobic part and NAD-binding site of the enzyme. The character of the structural changes in the hydrophobic part of the protein in diabetes and an increase in the enzymic activity are similar to that observed in normal aldolase after its interaction with NADH and are believed to be associated with the enhancement of the rigidity in the Trp-147 environment.     

Studies on the activity of aldolase from rabbit muscles in the presence of liposomes]

Electronmicroscopic studies have been made on the structure of liposomes obtained by the method of Bangham [13] with subsequent ultrasonic desintegration. The effect of muscle aldolase on the structure of liposomes was also investigated. Parallel studies were made on the effect of storage of liposomes upon the activity of aldolase. It was shown that liposomes obtained from chromatographically pure egg lecithin present discrete partially aggregated bodies, 1.000-3.000 A in size, composed by concentric layers, which have a dimension of approximately 40 A and periodicity of about 70 A. Interaction of these particles with the protein results into their desintegration and enlargement, this process being accompanied by the formation of a "fringe" at the edge of the particles. Aldolase activity in these systems in higher than in control. During storage of phosphatide-aqueous system, obtained by the metod of Bungenberg de Jong, activation of aldolase is gradually replaced by its inactivation.     

Dopamine transporter oligomerization: impact of combining protomers with differential cocaine analog binding affinities

Previous studies point to quaternary assembly of dopamine transporters (DATs) in oligomers. However, it is not clear whether the protomers function independently in the oligomer. Is each protomer an entirely separate unit that takes up dopamine and is inhibited by drugs known to block DAT function? In this work, human embryonic kidney 293 cells were co‐transfected with DAT constructs possessing differential binding affinities for the phenyltropane cocaine analog, [³H]WIN35,428. It was assessed whether the binding properties in co‐expressing cells capable of forming hetero‐oligomers differ from those in preparations obtained from mixed singly transfected cells where such oligomers cannot occur. A method is described that replaces laborious ‘mixing’ experiments with an in silico method predicting binding parameters from those observed for the singly expressed constructs. Among five pairs of constructs tested, statistically significant interactions were found between protomers of wild‐type (WT) and D313N, WT and D345N, and WT and D436N. Compared with predicted K_d values of [³H]WIN35,428 binding to the non‐interacting pairs, the observed affinity of the former pair was increased 1.7 fold while the latter two were reduced 2.2 and 4.1 fold, respectively. This is the first report of an influence of protomer composition on the properties of a DAT inhibitor, indicating cooperativity within the oligomer.

     

Comparative study of the structural characteristics of aldolase in rabbit muscles in normal states and in alloxan diabetes

It is shown that the activity of aldolase synthesized in rabbit muscles under diabetes is higher than that at normal state. This fact is probably a result of some structural alterations in NAD-binding site with Trp-291 and -311 in it which overlaps a considerable part of C-terminal region of the protein. The hydrophobic part of the enzyme containing Trp-147 under diabetes seems to remain unaltered. This consideration is based on the longwave shift in aldolase fluorescence lambda max (from 320 to 324 nm) under this pathology, suggesting a transition of Trp-291 and -311 into more polar environment and is confirmed by the disappearance of the difference in lambda max in the NADH presence. The NADH-originated shift in lambda max position for the both proteins ended at the same wave-length at 314 nm. The position of lambda max at 324 nm resulting from possible structural modification of NAD-binding site under diabetes correlates with an increase in the Stern-Volmer quenching constant value (from 4359 to 7500 M-1 for aldolase under normal and diabetic states, respectively). These quenching data evidence in favour of the suggestion on the existence of two classes of tryptophanyls in the aldolase molecule.     

Subunit structure of rabbit brain aldolase

Rabbit brain contains a mixture of aldolase A (muscle type) and aldolase C (brain type), present largely as the hybrid forms A₃C, A₂C₂, and AC₃, with smaller amounts of the homopolymers A₄ and C₄. We have developed new procedures for the isolation of the A-C hybrid set and the aldolase C subunits and compared the structure of these subunits with those of aldolase A. The two isoenzymes differ significantly in amino acid composition, but each contains three methionine residues per subunit and yields four peptides on cleavage with cyanogen bromide. The three methionine residues appear to occupy similar positions in the polypeptide chains but the molecular weight of the aldolase C subunit is only 37,000, approximately 10% smaller than that of the subunit of aldolase A. The difference is attributable to two or more deletions, totaling 30–40 amino acid residues, in two of the four BrCN peptides. The deletions include two of the buried cysteine residues that are located in the center of the polypeptide chain in aldolase A; these residues in aldolase A are, therefore, not involved in the contacts between the subunits in the tetramer. Aldolase C also lacks several of the histidine residues that are located near the active-site lysine residue of aldolase A, thus excluding these residues from participation in the catalytic mechanism.     

The NADP binding site on rabbit muscle aldolase

Rabbit muscle aldolase binds NADPH with a 1:1 stoichiometry and with a dissociation constant 18 microM. Three sites of the dinucleotide are involved in the binding: the adenosyl diphosphate moiety, the nicotinamide-ribose, and the nicotinamide ring. These data show the existence of a specific dinucleotide binding site in the aldolase molecule.     

Radiation inactivation of rabbit muscle aldolase.

Pulse radiolysis and steady-state X-radiolysis have been used to investigate the radiation inactivation of aldolase from rabbit muscle. Both eaq-and OH readily react with aldolase, and contribute to inactivation. The radical anions (CNS)2-and (Br)2-react with aldolase at neutral pH. The progressive addition of alkali results in an increase in the second-order rate constants, with an apparent pK approximately 10 +/- 0-3, and with the formation of an unstable intermediate, lambdamax approximately 400 nm resembling a phenoxyl radical. Steady-state radiolysis in the presence of (CNS)2-and (Br)2- at alkaline pH results in increased aldolase inactivation, with a pK of enzyme inactivation similar to that observed for reaction of the radical anions. We propose that a reaction of the radical anoins with tyrosine residues accounts for the resultant inactivation.     

Modification of rabbit muscle aldolase in Vivo and in Vitro

Rabbit muscle aldolase in situ appears to undergo several modification reactions. One of these, specific deamidation of an asparagine residue near the COOH-terminus, appears to account for the presence of two types of subunits in the enzyme isolated from the muscle of adult rabbits. Evidence for a second modification is the presence of approximately one equivalent of organic phosphorus in the crystalline enzyme preparations. The presence of this phosphate group may be related to the incomplete release of COOH-terminal tyrosine residues from the enzyme protein with carboxypeptidase. Two reactions with substrate, both leading to the incorporation of organic phosphorus, have been demonstrated in vitro. A reaction with glyceraldehyde 3-phosphate or erythrose 4-phosphate leads to loss of catalytic activity and change in the susceptibility of COOH-terminus to carboxypeptidase. The other reaction, with fructose 1,6-diphosphate at low concentration, does not affect the activity of the enzyme, nor its susceptibility towards the action of carboxypeptidase. Either or both of these may be related to the changes which appear to occur during the life of the enzyme in vivo.