Enrique Palacián

Dicarboxylic acid anhydrides as dissociating agents of protein-containing structures

Dissociation of protein-containing structures by modification of protein amino groups with dicarboxylic acid anhydrides is a mild procedure which, in some cases, offers advantages over treatment with alternative dissociating agents, such as urea, guanidine hydrochloride, detergents, high ionic strength, and extremes of pH: In addition to dissociating multimeric proteins and protein aggregates, dicarboxylic acid anhydrides are effective dissociating agents for membrane-bound proteins and nucleoprotein particles. With most dicarboxylic acid anhydrides reviewed, the introduced reagent residues can be eliminated under moderate acid conditions, which allows the purification of unmodified individual components, and the use of disassembly-reconstitution systems valuable for investigating the structural and functional roles played by the individual components of complex particles:Each reagent can be suitable for a particular purpose, depending on the required specificity of the modification and stability of the modified groups: The stability of the acylated amino groups ranges from the very stable succinylated amino groups to the very labile acylation obtained with dimethylmaleic anhydride: Between these extremes, the stability of the modified amino groups decreases stepwise in the following order: maleic, exo-cis-3,6-endoxo-Δ4-tetrahydrophthalic, citraconic, and 3,4,5,6-tetrahydrophthalic anhydride. With respect to the selectivity of the produced modification, little or no modification of hydroxyamino acid and cysteine residues has been observed with dimethylmaleic, exo-cis-3,6-endoxo-Δ4-tetrahydrophthalic, and 3,4,5,6-tetrahydrophthalic anhydrides: With the other reagents, the extent of modification of hydroxyamino acid residues increases in the order citraconic, maleic and succinic anhydride: Citraconic and maleic anhydrides can produce irreversible modification of cysteine residues, the reactivity of sulfhydryl groups being higher with maleic anhydride:

Effects of temperature and pH on the regeneration of the amino groups of ovalbumin after modification with citraconic and dimethylmaleic anhydrides

The reagents citraconic and dimethylmaleic anhydrides modify the amino groups of proteins in a reversible way, the modified amino groups being regenerated at moderate acid pH. To use these reagents efficiently it is important to know the stabilities of the modifed groups under different experimental conditions. We have studied the kinetics of deacylation of ovalbumin amino groups modified with citraconic and dimethylmaleic anhydrides, under different conditions of temperature (0-40 degrees C) and pH (4-8). The deacylation of the modified groups follows pseudo-first-order kinetics under all experimental conditions studied. For both reagents, the dependence of the rate of deacylation on temperature obeys the Arrhenius equation, and the logarithm of the apparent deacylation constant shows a linear dependence on pH. From the experimental data, equations have been obtained for both reagents relating the deacylation constant with temperature and pH. These equations allow the calculation of the deacylation constant and the half-life of the modified groups for any conditions of temperature and pH within the experimental intervals studied.

Interaction of RNA polymerase II with acetylated nucleosomal core particles

Chemical acetylation of nucleosomal cores is accompanied by an increase in their efficiency as in vitro transcription templates. Low amounts of acetic anhydride cause preferential modification of the amino-terminal tails of core histones. Modification of these domains, which causes moderate structural effects, is apparently correlated with the observed stimulation of RNA synthesis. In contrast, extensive modification of the globular regions of core histones, which is accompanied by a large structural relaxation of the particle, causes little additional effect on transcription. Acetylation of the amino-terminal domains of histones might stimulate transcription by changing the interaction of the histone tails with components of the transcriptional machinery.

Partial reconstitution of 60S ribosomal subunits from yeast

SummaryRibosomal 60S subunits active in polyphenylalanine synthesis can be reconstituted from core particles lacking 20–40% of the total protein. These core particles were obtained by treatment of yeast 60S subunits with dimethylmaleic anhydride, a reagent for protein amino groups. Upon reconstitution a complementary amount of split proteins is incorporated into the ribosomal particles, which have the sedimentation coefficient of the original subunits. Ribosomal protein fractions obtained by extraction with 1.25 M NH4Cl, 4 M LiCl, 7 M LiCl, or 67% acetic acid, are much less efficient in the reconstitution of active subunits from these core particles than the corresponding released fraction prepared with dimethylmaleic anhydride. Attempts to reconstitute active subunits from protein-deficient particles obtained with 1.25 M NH4Cl plus different preparations of ribosomal proteins, including the fraction released with dimethylmaleic anhydride, were unsuccessful. Therefore, under our conditions, of the disassembly procedures assayed only dimethylmaleic anhydride allows partial reconstitution of active 60S subunits.

Dissociation of nucleosomal particles by chemical modification. Equivalence of the two binding sites for H2A.H2B dimers

Resumen del poster presentado al 50th Inner Ear Biology Workshop, celebrado en Alcala de Henares-Madrid (Espana) del 10 al 13 de septiembre de 2013.Resumen del trabajo presentado al 15o Congreso Nacional de la Sociedad Espanola de Neurociencia (SENC) celebrado en Oviedo del 25 al 27 de septiembre de 2013.Resumen del poster presentado al CIBERDEM Annual Meeting, celebrado en Cerdanyola del Valles, Barcelona (Espana) del 11 al 13 de mayo de 2016.-- et al.Resumen del trabajo presentado al XXXVIII Congreso de la Sociedad Espanola de Ciencias Fisiologicas (SECF), celebrado en Zaragoza del 13 al 16 de septiembre de 2016.Poster presentado en el XI European Meeting on Glial Cells in Health and Disease, celebrado los dias 3 al 6 de julio de 2013 en Berlin (Alemania)Memoria presentada para optar al grado de Doctor por la Licenciada en Biologia Angela Prieto Folgado y realizada en el Instituto de Investigaciones Biomedicas Alberto Sols.La realizacion de este trabajo ha sido posible gracias a la financiacion otorgada por el FIS al proyecto de investigacion 96/1803.Grant Funding Source: Supported by the Fondo de Investigaciones Sanitarias (PI0011406) to MF.The chemotherapeutic study of a limited series of steroidal sapogenins from several endemic species of the flora of the Canary Islands is presented here. On the whole, they possess a very weak antibacterial activity, a slight antifungal effect and one of them, vespertilin, displays interesting cytostatic activity (ID50 = 5 micrograms/ml). A pharmacodynamic screening carried out on this product mainly revealed very slight toxicity, antihistaminic activity and a light tranquilizing effect. The data obtained justify further research.The purpose of this study was to characterize the role of ions other than Ca2+ in hepatic responses to alpha 1-adrenergic stimulation. We report that the alpha 1-adrenoreceptor activation of hepatic functions is accompanied by extracellular acidification and an increase in intracellular pH. These effects are dependent on extracellular Na+ concentration and are inhibited by the Na+/H+ antiporter blocker 5-(N-ethyl-N-isopropyl) amiloride under conditions that preclude antagonistic effects on agonist binding. Thus, the activation of plasma membrane Na+/H+ exchange is an essential feature of the hepatic alpha-adrenoreceptor-coupled signaling pathway. The following observations indicate that the sustained hepatic alpha 1-adrenergic actions rely on a functional coupling between the plasma membrane Na+/H+ and Na+/Ca2+ exchangers, resulting in the stimulation of Ca2+ influx. 1) Inhibition of the Na+/K(+)-ATPase does not prevent the alpha 1-adrenergic effects. However, alpha 1-adrenoreceptor stimulation fails to induce intracellular alkalinization and to acidify the extracellular medium in the absence of extracellular Ca2+. 2) A non-receptor-induced increase in intracellular Na+ concentration, caused by the ionophore monensin, stimulates Ca2+ influx and increases vascular resistance. 3) Inhibition of Na+/Ca2+ exchange prevents, in a concentration-dependent manner, most of the alpha 1-agonist-induced responses. 4) The actions of Ca(2+)-mobilizing vasoactive peptide receptors or alpha 2-adrenoreceptors, which produce neither sustained extracellular acidification nor release of Ca2+, are insensitive to Na+/H+ exchange blockers.Poster presentado en la VII Reunion Anual de la Red Tematica de Investigacion Cooperativa en Cancer (RTICC), celebrada en Salamanca el 24 de septiembre de 2014Resumen del trabajo presentado al VI Meeting de la Red Espanola de Canales Ioniocs (RECI), celebrado en Santiago de Compostela del 6 al 8 de septiembre de 2017.Tesis Doctoral presentada por Laura Jimenez Perez para optar al grado de doctor por la Universidad de Valladolid, Departamento de Bioquimica y Biologia Molecular y FisiologiaPoster presentado en la VII Reunion Anual de la Red Tematica de Investigacion Cooperativa en Cancer (RTICC), celebrada en Salamanca el 24 de septiembre de 2014Resumen del trabajo presentado al XXXXVIII Congreso de la Sociedad Espanola de Bioquimica y Biologia Molecular (SEBBM), celebrado en Valencia del 7 al 10 de septiembre de 2015.Esta Tesis Doctoral fue realizada en el Centro Andaluz de Biologia del Desarrollo por la licenciada Briseida Beli Cacho Valadez para optar al grado de Doctor por la Universidad Pablo de Olavide.Rat liver S-adenosylmethionine (AdoMet) synthetase appears as high-M(r) (tetramer) and low-M(r) (dimer) forms. Both are inhibited in the presence of GSSG at pH 8. The calculated Ki values are 2.14 and 4.03 mM for the high- and low-M(r) forms, respectively. No effect on enzyme activity was observed in the presence of GSH, but modulation of inhibition by GSSG can be obtained by addition of GSH. At a total glutathione concentration (GSH + GSSG) of 10 mM, a KOX of 1.74 was calculated for the high-M(r) form, whereas this constant was 2.85 for the low-M(r) AdoMet synthetase. No incorporation of [35S]GSSG was observed in either of the enzyme forms, and inhibition of enzyme activity was correlated with dissociation of both AdoMet synthetases to a monomer. The data obtained in the presence of GSSG seem to suggest that oxidation leads to the formation of an intrasubunit disulfide. The possible regulation of AdoMet synthetase activity by the GSH/GSSG ratio is discussed, as well as its in vivo significance.Trabajo presentado en el XI Simposi de Neurobiologia: Future technical advances, organizado por la Socitat Catalana de Biologia, en Barcelona, los dias 12 y 13 de noviembre de 2018El estudio de la relacion entre componentes de la dieta y la salud/enfermedad utiliza metodos de valoracion de la ingesta dietetica, del estatus nutricional y de marcadores de funcion o de efecto. En concreto, en el estudio de los carotenoides y la salud ocular, interesa el estudio de dos carotenoides sin actividad provitamina A, la luteina y la zeaxantina, por su posible papel en la optimizacion de la funcion visual y en la prevencion de enfermedades cronicas asociadas a la edad, y de tres carotenoides con actividad provitamina A: -caroteno, -caroteno y -criptoxantina, por ser precursores de retinol, nutriente del que depende el ciclo visual para una vision normal. En el presente trabajo se ha llevado a cabo el estudio de los carotenoides de la dieta mas relevantes para la salud ocular humana considerando de forma simultanea parametros relacionados con la ingesta, el estatus y la funcion visual, asi como diversas variables que pueden modificar el estatus nutricional, como son la concentracion de lipidos en sangre, y la bioaccesibilidad de los carotenoides a partir de alimentos de amplio consumo...Fetal rat hepatocytes treated with transforming growth factor beta (TGF-beta) die by apoptosis. However, a subpopulation of them survives and undergoes an epithelial mesenchymal transition (EMT). This transition also occurs upon incubation with fetal bovine serum. We have isolated the subpopulations that undergo EMT (TGF-beta-treated-fetal hepatocytes: TbetaT-FH; serum-treated-fetal hepatocytes: ST-FH) and show that they present high levels of vimentin and Snail expression and lack cytokeratin 18 and E-cadherin. Both TbetaT-FH and ST-FH cells require mitogens to grow and maintain the response to TGF-beta in terms of growth inhibition. However, they lack differentiation markers such as the liver-enriched transcription factors hepatocyte nuclear factor 4 (HNF-4) or HNF-1alpha and express the progenitor marker OV-6. Interestingly, the EMT process confers them resistance to the apoptotic effect of TGF-beta, with cells showing higher levels of active AKT and Bcl-x(L) than fetal hepatocytes. In summary, these cells are refractory to the apoptotic effects of TGF-beta, showing characteristics of liver progenitors and of some hepatocellular carcinoma cells.Memoria de tesis presentada por Luis Vazquez Fonseca, Licenciado en Bioquimica para optar al grado de Doctor. Esta Tesis Doctoral ha sido realizada bajo el programa de doctorado de Biotecnologia y Tecnologia Quimica en el grupo de investigacion del CIBERER U729 en el Centro Andaluz de Biologia del Desarrollo, Area de Biologia Celular del Departamento de Fisiologia, Anatomia y Biologia Celular de la Universidad Pablo de Olavide y bajo la direccion del Dr. Carlos Santos Ocana y el Dr. Placido NavasResumen del poster presentado al Joint FEPS & XXXVI Spanish Physiological Society Congress (Sociedad Espanola de Ciencias Fisiologicas) celebrado en Santiago de Compostela (Espana) del 8 al 11 de septiembre de 2012.Poster presentado al 17o Congreso Nacional de la Sociedad Espanola de Neurociencia, celebrado en Alicante del 27 al 30 de septiembre de 2017.The mutations at the bithorax locus produce a transformation of anterior haltere into anterior wing. The bx1 allele presents unusual features when compared with other bx alleles. The phenotype of bx1 homozygotes is temperature sensitive but only with regard to the distal and not to the proximal transformation, thus suggesting two different components in the bithorax transformation. The phenotype of bx1 homozygotes is stronger than that of bx1 over the deletion of the gene, suggesting a trans interaction of the bx1 chromosomes which results in mutual partial inactivation. We show by temperature shift and clonal analysis experiments that the decision on whether to differentiate haltere or wing structures is taken at the end of the proliferation period of the mutant disc.Poster presentado al XXXVII Congreso de la Sociedad Espanola de Bioquimica y Biologia Molecular, celebrado en Granada del 9 al 12 de septiembre de 2014.Poster presentado al XXVII Congreso Nacional de la Asociacion Espanola de Genetica Humana celebrado en Madrid del 10 al 12 de abril de 2013.Poster presentado al XXXVII Congreso de la Sociedad Espanola de Bioquimica y Biologia Molecular, celebrado en Granada del 9 al 12 de septiembre de 2014.Poster presentado en el XI European Meeting on Glial Cells in Health and Disease, celebrado los dias 3 al 6 de julio de 2013 en Berlin (Alemania)Resumen del trabajo presentado al Spanish Society of Biochemistry and Molecular Biology (SEBBM), celebrado en Madrid del 16 al 19 de julio de 2019.Poster presentado en el XII European Meeting on Glial Cells in Health and Disease, celebrado los dias 15 a 18 de julio de 2015 en Bilbao (Espana)Trabajo presentado en el XL Congreso de la Sociedad Espanola de Bioquimica y Biologia Molecular. FEBS3+1st Joint Meeting of the French-Portuguese-Spanish Biochemical and Molecular, celebrado en Barcelona (Espana), del 23 al 26 de octubre de 2017Resumen del poster presentado al Joint FEPS & XXXVI Spanish Physiological Society Congress (Sociedad Espanola de Ciencias Fisiologicas) celebrado en Santiago de Compostela (Espana) del 8 al 11 de septiembre de 2012.Trabajo presentado en el XII GEIRLI Meeting: New trends in redox biology: a multidisciplinary approach, celebrado en Barcelona (Espana), los dias 4 y 5 de julio de 2019Treatment of nucleosomal particles with dimethylmaleic anhydride, a reagent for protein amino groups, is accompanied by a biphasic release of histones H2A plus H2B; one H2A.H2B dimer is more easily released than the other. This behavior allows the preparation of nucleosomal particles containing only one H2A.H2B dimer, which were complemented with 125I-labeled H2A.H2B. These reconstituted particles, which contain one labeled and one unlabeled H2A.H2B dimer, were treated with the amount of reagent needed to release one of the two H2A.H2B dimers. Radioactivity was equally distributed between residual particles and released proteins, which is consistent with equivalent binding sites in the nucleosomal particle for H2A.H2B dimers, rather than with intrinsically different sites. The asymmetric release of H2A.H2B dimers would be caused by a change in the binding site of one dimer following the release of the other. This behavior might be related to the structural dynamics of nucleosomes.Resumen del trabajo presentado al European Society of Cardiology (ESC) Congress, celebrado en Barcelona (Espana) del 26 al 30 de agosto de 2017.Resumen del poster presentado al 49th European Association for the Study of Diabetes Annual Meeting, celebrado en Barcelona (Espana) del 23 al 27 de septiembre de 2013.-- et al.Trabajo doctoral realizado por Da Rebeca Lapresa Ruiz de Gauna, para optar al grado de doctor por la Universidad de Salamanca.Rationale: Several animal models have been developed to study acute lung injury (ALI); however the majority of these studies are focused on different mechanisms within the acute phase. These models do not allow studying the mechanisms in the later phases or testing any possible long-term treatment. The aim of this study was to develop an experimental ALI model simulating bronchial aspiration of gastric contents with bacterial superinfection with alveolar epithelial damage persisting over time. Methods: Sprague-Dawley rats (200-250g) were anesthetized with isofluorane. ALI was induced by intratracheal instillation of HCl (1 µl/g, 0.1 mol/L pH=1.4) followed by instillation of LPS from Escherichia coli O55:B5 (0, 10, 20, 30 or 40µg/g b.w.) two hours later. Control rats were treated with intratracheal instillations of saline. After 72h, the animals were sacrificed and bronchoalveolar lavage fluid (BALF) was sampled for further analysis of total protein concentration by bicinchoninic acid method. Results: At 72 h, rats suffered a significant loss of weight proportional to the administered dose of LPS (5.6% with 10µg/g b.w, 12.6% with 20µg/g b.w, 14.2% with 30µg/g b.w and 17.7% with 40µg/g b.w). Control rats gained in weight at 72h. LPS at 10, 20, 30 and 40µg/g b.w induced a 1.7, 2.5, 2.9 and 3.4 fold increase in total protein concentration in BAL fluid, respectively, reflecting a substantial increase proportional to the LPS dose. Conclusion: The degree of weight loss and the increase of total protein concentration in BAL fluid in the current model may reflect disease severity and progression. This model would be useful in future for new therapeutical options. Grant acknowledgements: FIS-PI12/02548 and Fundacio Parc Tauli.Resumen del trabajo presentado al European Respiratory Society (ERS) International Congress, celebrado en Paris (Francia) del 15 al 19 de septiembre de 2018.Resumen del trabajo presentado a las 5as Jornadas de Formacion del CIBERES celebradas en Bunyola (Mallorca) del 18 al 19 de octubre de 2012.Resumen del poster presentado al Joint FEPS & XXXVI Spanish Physiological Society Congress (Sociedad Espanola de Ciencias Fisiologicas) celebrado en Santiago de Compostela (Espana) del 8 al 11 de septiembre de 2012.Resumen del trabajo presentado al XIII Congreso de la Sociedad Espanola del Dolor, celebrado en Pamplona del 2 al 4 de junio de 2016.This work was supported by grants FIS-01/1048 and FIS-02/1199 from the Fondo de Investigacion Sanitaria and grant SA-087/01 from Junta de Castilla y Leon.Resumen del poster presentado al Joint Meeting of the American Physiological Society and the Physiological Society, celebrado en Dublin (Irlanda) del 29 al 31 de julio de 2016.Trabajo presentado al 5th International Conference on Phospholipase A2 Mediated Signaling in Translational Medicine celebrado en New Orleans (US) del 20 al 21 de mayo de 2013.Tesis Doctoral presentada por Rebeca Torres Merino para optar al grado de Doctora por la Universidad de Valladolid, Facultad de Medicina: Dpto. de Bioquimica y Biologia Molecular y Fisiologia.Poster presentado al Annual Meeting of the Association for Research in Vision and Ophthalmology (ARVO), celebrado en Seattle, Washington (US) del 1 al 5 de mayo de 2016.Resumen del trabajo presentado al 63rd Annual Meeting Biophysical Society, celebrado en Baltimore, Maryland (USA) del 2 al 6 de marzo de 2019.Poster presentado al XXXVII Congreso de la Sociedad Espanola de Bioquimica y Biologia Molecular, celebrado en Granada del 9 al 12 de septiembre de 2014.Resumen del poster presentado a la 5th Conference on Advances in Molecular Mechanisms Underlying Neurological Disorders (Joint conference of the European Society for Neurochemistry and the Biochemical Society) en la University of Bath (UK) del 23 al 26 de junio de 2013.-- Tambien presentado al 15o Congreso Nacional de la Sociedad Espanola de Neurociencia (SENC) celebrado en Oviedo del 25 al 27 de septiembre de 2013.Resumen del trabajo presentado al XXXVI Congreso de la Sociedad Espanola de Bioquimica y Biologia Molecular celebrado en Madrid del 4 al 6 de septiembre de 2013.Resumen del trabajo presentado a la 5th Conference on Advances in Molecular Mechanisms Underlying Neurological Disorders (Joint conference of the European Society for Neurochemistry and the Biochemical Society) en la University of Bath (UK) del 23 al 26 de junio de 2013.Resumen del poster presentado al XXVIII Congreso Nacional de la Sociedad Espanola de diabetes, celebrado en Bilbao del 20 al 22 de abril de 2016.SAF2016-77703-C2-2-R of the Ministerio de Economia y Competitividad, Spain and the European Regional Development Fund (ERDF); AGAUR 2017-SGR106 and the CERCA Programme of the Generalitat de Catalunya; C. Sanfeliu belong to Group 05 of CIBER Epidemiologia y Salud Publica (CIBERESP) of the Instituto de Salud Carlos III, Ministerio de Sanidad y Consumo, Spain

Protein-deficient ribosomal particles obtained by reversible modification with dimethylmaleic anhydride

Abstract Preparation of protein-deficient ribosomal particles from Escherichia coli ribosomes by reversible modification of protein amino groups with dimethylmaleic anhydride ( J. A. Pintor-Toro, D. Vazquez, and E. Palacian, 1979, Biochemistry18, 3219 ) is accompanied by degradation of r-RNA and reagent-independent inactivation. Alternative conditions to regenerate the modified amino groups have been found, which reduce the time needed to prepare the ribosomal “cores” from 9 to 3 days, and prevent RNA degradation and inactivation. The ribosomal particles obtained from 70 S ribosomes and 50 S subunits by this modified procedure show no extensive degradation of RNA and very little reagent-independent inactivation, which allow good recovery of the polypeptide synthesizing activity when incubated with the corresponding split proteins.

Transcription of mononucleosomal particles acetylated in the presence of n-butyrate.

Although a correlation between chemical acetylation of the amino-terminal tails of core histones and stimulation of RNA synthesis has been reported for nucleosomal core particles (Piñeiro et al. (1991) Biochem. Biophys. Res. Commun. 177: 370), no differences in transcription are detected between acetylated and nonacetylated mononucleosomal particles obtained from HeLa cells in the presence and absence of n-butyrate. Apparently, the lysine residues modified in the presence of n-butyrate are not the same responsible for the observed acetylation-induced transcription. The acetylation obtained with n-butyrate might be significantly different from that present in transcriptionally active chromatin.

Dissociation of the protein components from chromatin by reversible modification with dimethylmaleic anhydride.

SummaryModification of calf thymus chromatin with the protein reagent dimethylmaleic anhydride is accompanied by dissociation of histones and non-histone proteins. Gel electrophoresis of the released proteins and of those bound to the residual chromatin showed that histone H1 is dissociated more easily than the core histones (H2A, H2B, H3 and H4). These are apparently released in the proportion in which they are present in chromatin. After regeneration of the modified amino groups by incubation at pH 6.0, the released proteins are able to bind to the residual chromatin, under two different sets of reconstitution conditions, to form nucleosome-like structures.

Succinylation of histone amino groups facilitates transcription of nucleosomal cores

Treatment of nucleosomal cores with succinic anhydride, which modifies preferentially the amino-terminal domains of core histones, takes place without dissociation of the particles. Low levels of modification, which cause small structural effects, are accompanied by substantial increases in the efficiency of the nucleosomal cores as in vitro transcription templates for RNA polymerase II. The transcriptional properties of the succinylated nucleosomal cores are similar to those of the acetylated particles (Piñeiro et al., (1991) Biochem. Biophys. Res. Commun. 177, 370-376), indicating that no specific blocking by acetyl residues is required to facilitate in vitro transcription. Moreover, to obtain a certain level of stimulation, a smaller number of groups has to be modified by succinic than by acetic anhydride.

Disassembly and reconstitution of yeast 60S ribosomal subunits

SummaryYeast 60S ribosomal subunits have been dissociated by reversible modification with dimethylmaleic anhydride. Treatment with 40 μmol reagent/ml releases 35% of the protein, producing core particles inactive in polyphenylalanine synthesis, which are totally or highly deficient in 17 different proteins. This preparation of residual particles recovers 45% of the original activity upon incubation with the released proteins. The reconstituted particles can be isolated by centrifugation without loss of activity, having the protein composition of the original subunits.