Spectroscopic study of trypsin, heat and triton X-100-induced denaturation of the chlorophyll-binding protein CP43

Trypsin-, heat- and Triton X-100-induced denaturation of CP43, the core antenna complex of photosystem II purified from spinach, has been investigated using absorption, fluorescence and circular dichroism spectroscopy. Triton X-100 was found to bring about considerable dissolution of pigments from the protein to the monomeric state in solution and destruction of the interactions among the chlorophyll, carotene and protein. Heat induced significant unfolding of the protein secondary structure and loss of excitonic interactions of the pigments, but no apparent dissolution of the pigments from CP43. Trypsin caused structural changes in the extrinsic part of the protein but no change of the native state of the pigments. Trypsin, heat and Triton X-100 treatments increased the light sensitivity of chlorophyll in CP43 to different extents. The results suggest that the protein and beta-carotene can protect the chlorophyll from light-induced destruction in CP43.     

Triton X-100在乙二醇中的胶体性质

表面活性剂在非水溶剂中聚集态的研究所见的报导与水体系相比要少得多．然而近年来对非水体系的研究日益增多．这是因为表面活性剂在非水溶剂中的应用日趋增加，但与水体系相反，对非水体系的性质了解甚少．对表面活性剂非水体系的研究还有助于对其聚集体的共溶剂效应有更深的认识．TritonX－100（以下简写为TX－100）是典型的非离子表面活性剂，在工业上有着广泛的应用．乙二醇在多醇中与水的化学结构最相近问，然而它却是水结构的破坏剂，加入少量的乙二醇会使水的冰点急剧下降．乙二醇又是蛋白质的变性溶剂．表面活性剂在乙二醇中的胶…     

Daunomycin binding to detergent micelles: a model system for evaluating the hydrophobic contribution to drug-DNA interactions

The interaction of daunomycin with sodium dodecyl sulfate and Triton X-100 micelles was investigated as a model for the hydrophobic contribution to the free energy of DNA intercalation reactions. Measurements of visible absorbance, fluorescence lifetime, steady-state fluorescence emission intensity, and fluorescence anisotropy indicate that the anthraquinone ring partitions into the hydrophobic micelle interior. Fluorescence quenching experiments using both steady-state and lifetime measurements demonstrate reduced accessibility of daunomycin in sodium dodecyl sulfate micelles to the anionic quencher iodide and to the neutral quencher acrylamide. Quenching of daunomycin fluorescence by iodide in Triton X-100 micelles was similar to that seen with free daunomycin. Studies of the energetics of the interaction of daunomycin with micelles by fluorescence and absorbance titration methods and by isothermal titration calorimetry in the presence of excess micelles revealed that association with sodium dodecyl sulfate and Triton X-100 micelles is driven by a large negative enthalpy. Association of the drug with both types of micelles also has a favorable entropic contribution, which is larger in magnitude for Triton X-100 micelles than for sodium dodecyl sulfate micelles. The thermodynamic profile for the interaction of daunomycin with both types of micelles is characteristic of the "nonclassical" hydrophobic effect. The enthalpy for the interaction of daunomycin with sodium dodecyl sulfate micelles increases nonlinearly with temperature, indicating a positive (and temperature dependent) heat capacity change. The binding isotherm for daunomycin association with sodium dodecyl sulfate micelles was cooperative, with a Hill coefficient of 1.6. The cooperative behavior and the positive heat capacity change suggest that the drug alters micelle size or imposes order on the hydrocarbon interior of the micelle.     

Light- and heat-induced denaturation of photosystem II core-antenna complexes CP43 and CP47

Light- and heat-induced denaturation of the core-antenna complexes of Photosystem II, CP43 and CP47, purified from spinach, has been investigated using absorption, fluorescence and circular dichroism (CD) spectroscopy. Light is found to bring about considerable bleaching of chlorophyll a but no apparent change in the protein secondary structure, while heat induces significant unfolding of the protein secondary structure but no apparent destruction of the chlorophyll a molecule in the two antenna complexes. Both the destruction of chlorophyll a by light and the denaturation of the protein conformation by heat cause the loss of excitonic interaction of chlorophyll a in CP43 and CP47, as measured by visible CD activity. Light induces a larger decrease of the chlorophyll a fluorescence and the CD activity of CP47 than that of CP43, indicating that the native state of chlorophyll a of CP47 is more sensitive to light than that of CP43. The main thermal transitions of protein secondary structure occur at 50°C for CP43 and 63°C for CP47, while the half-loss of chlorophyll a excitonic interaction during heating occurs at 45°C for CP43 and 60°C for CP47, suggesting that CP47 is more thermally stable than CP43.     

Adsorptive immobilization of intestinal brush border membrane on triton X-100-substituted sepharose 4B

Triton X-100-substituted Sepharose 4B (Sepharose-TX) was used for adsorptive immobilization of intestinal brush border membrane using lactose-phlorizin hydrolase as a representative membrane enzyme. Limited heating of membrane preparations was found to enhance binding. This enhancement is concluded to be owing to a greater availability of the hydrophobic sites, as also confirmed by the 1-anilino-8-naphthalene sulfonate fluorescence studies, for interaction with Triton X-100 moieties on the support. The immobilized preparations obtained by this procedure were found useful in hydrolysis of lactose, involving lactose-phlorizin hydrolase, in continuous operations. It is suggested that the approach may be of general utility for immobilization of biologic membranes by interaction of their extramembrane structures using supports with appropriate hydrophobic groups.     

Period-four Modulation of Photosystem II Primary Quinone Acceptor (QA) Reduction/Oxidation Kinetics in Thylakoid Membranes

Photosystem II (PSII), a multiprotein complex mainly coded by the chloroplast genome in higher plants and algae, contains the oxygen-evolving complex with four manganese atoms responsible for the oxidation of water. After each absorption of a light quantum by pigment molecules in the light harvesting complexes of PSII, the Mn cluster advances in its oxidation states denoted from S₀ to S₄. The S₄ state decays to S₀ in the dark with the concurrent release of molecular oxygen. Therefore, the oxygen production in PSII exposed to successive single turnover excitations follows a period-four oscillation pattern. The intensity of chlorophyll a fluorescence of PSII is also known to be influenced by the oxidation state of the Mn cluster. In the present work, fluorescence induction kinetics was measured in isolated thylakoids with various initial S-state populations settled by preflashes. The shape of the fluorescence induction traces was strongly affected by preflashes. O-J and J-I phases of the induction followed a period-four oscillation pattern. The results indicate that these changes reflect the influence of the oxidation rate of the Mn cluster on the reduction/oxidation kinetics of the primary quinone acceptor (Q_A) of PSII.     

STUDIES OF SODIUM TAUROCHOLATE MICELLES USING FLUORESCENT PROBE MOLECULES

Abstract Micelles formed by sodium taurocholate (NaTC) and mixed micelles formed by NaTC with detergents (SDS, reduced Triton X-100 and CTAC) were studied with fluorescent probes. Pyrene was used as an indicator of the polarity of the micellar binding site by comparison of the fluorescence spectra and vibronic band intensity ratios of pyrene in the different systems. Perylene was used as a fluorescence polarization probe to study the rigidity of the NaTC and mixed micelles. The fluorescence lifetime of perylene in the different systems was also measured. Results of the studies were compared with measurements of the probes in cyclohexane, ethanol and aqueous beta-cyclodextrin. Perylene was found to be more rigidly bound in the NaTC micelles than in the detergent micelles. Insertion of small amounts of reduced Triton X-100 into the NaTC micelles appears to increase the rigidity. The binding sites of NaTC and CTAC have similar polarities, and are more polar than those of SDS and reduced Triton X-100. Insertion of any of the detergents into the NaTC micelle decreases the polarity of the binding site, possibly by reducing the penetration of water into the micelle.     

Triton X-100对血红蛋白/利巴韦林/H2O体系中血红蛋白性质和药物释放的影响

通过紫外光谱、荧光光谱、zeta电位、电导率、高效液相色谱和影像分析等方法研究了Triton X-100对血红蛋白/利巴韦林/H2O体系中血红蛋白性质和药物控制释放的影响. 研究结果表明, 随着Triton X-100浓度的增大, 荧光强度、荧光偏振、zeta电位和蛋白的形貌均发生较大的变化, Triton X-100能使增溶定位在蛋白表面中的利巴韦林逐渐游离出来. 当Triton X-100浓度大于1×10^-5 mol·L-1 时, Triton X-100 与血红蛋白的作用占主导地位, 血红蛋白开始明显变性. 少量Triton X-100能保护蛋白免受药物的影响.     

曙红Y-Triton X-100疏水性氢键纳米微粒的吸收、荧光及共振瑞利散射光谱及其分析应用

在pH2.4～2.8的酸性介质中,曙红Y分子(H2L)取代水分子而与Triton X-100形成氢键缔合物.该疏水性的氢键缔合物,在水相的"挤压"作用和范德华力的作用下,能进一步聚集形成纳米微粒.此时将引起吸收光谱的变化和荧光猝灭,并导致共振瑞利散射(RRS)显著增强,为建立褪色分光光度法、荧光猝灭法和共振瑞利散射法测定Triton X-100创造了条件.三种方法均有较高的灵敏度.其中以RRS法灵敏度最高,对于Triton X-100的检出限为20.6ng/mL.本文研究了曙红Y与Triton X-100相互作用的适宜条件和对吸收、荧光和RRS光谱的影响.考察了共存物质的影响,表明方法有良好的选择性.发展和建立了灵敏、简便、快速测定Triton X-100的分光光度、荧光猝灭法和RRS新方法.文中还结合红外光谱、透射电子显微镜技术和量子化学方法对曙红Y-Triton X-100氢键缔合物及纳米微粒的形成以及对相应的光谱特性的影响进行了讨论,并研究了方法在环境分析中的应用.     

Absorption, fluorescence and resonance Rayleigh scattering spectra of hydrophobic hydrogen bonding of eosin Y/Triton X-100 nanoparticles and their analytical applications

In a weak acidic medium (pH 2.4–2.8), eosin Y molecules (H₂L) could replace water molecules to associate with Triton X-100 to form hydrophobic hydrogen bonding complexes. These complexes could further aggregate to form nanoparticles through the squeezing action of the water phase and Van Der Waals force, resulting in changes in the absorption spectrum and fluorescence quenching of EY as well as the significant enhancement of resonance Rayleigh scattering. This enables the sensitive determination of Triton X-100 using the fading spectrophotometry, fluorescence quenching method and RRS method. Among them, the RRS method shows the highest sensitivity with a detection limit of 20.6 ng mL^?1 for Triton X-100. The optimum experimental conditions and factors that affect the absorption, fluorescence and RRS spectra were tested. The effects of coexisting substances were investigated and the results showed good selectivity. Based on these results, new spectrophotometric methods, fluorescence quenching method and RRS method for the determination of Triton X-100, were established. The hydrogen bonding association of eosin Y with Triton X-100 and the formation of nanoparticles as well as their effects on related spectral characteristics were discussed utilizing infrared, transmission electron microscope technique and quantum chemical method.     

Effects of Triton X-100 on Properties of Hemoglobin and Controlled Release of Drug in Hemoglobin/Ribavirin/H2O System

Effects of Triton X-100 on the properties of hemoglobin (Hb) and on the controlled release of ribavirin were studied using the methods of UV-Vis spectrum, fluorescence spectrum, zeta potential, conductivity, high-performance liquid chromatographic (HPLC), and image morphology in Hb/ribavirin/H₂O system. With the increase of concentration of Triton X-100 in the system, the intrinsic fluorescence intensity, synchronous fluorescence intensity, fluorescence polarization, zeta potential, and morphology of Hb all changed gradually, and the ribavirin located on the Hb surface was dissociated and released out. When the concentration of Triton X-100 was higher than 1×10⁻⁵ mol·L⁻¹, the stronger interaction of Triton X-100 with Hb was predominant. Hb was unfolded and denaturized. A little Triton X-100 can protect Hb from the effects of ribavirin.     

Thermodynamic insights into the binding of Triton X-100 to globular proteins: a calorimetric and spectroscopic investigation

The interaction of the nonionic surfactant Triton X-100 (TX-100) with two proteins (bovine serum albumin (BSA) and alpha-lactalbumin (alpha-LA)) has been investigated by using a combination of differential scanning calorimetry, isothermal titration calorimetry, and fluorescence and circular dichroism spectroscopies. All of the calorimetric transitions in BSA were partially reversible, while being two-state and reversible in the case of alpha-LA. TX-100 molecules do not reduce the thermal stability of the protein in the monomeric form. However, in the micellar form the protein might become thermally destabilized by the micelles depending upon the nature of the protein. Isothermal titration calorimetry has been used to demonstrate that TX-100 binds to BSA at two sets of sites with 4:1 stoichiometry in each case. The van't Hoff enthalpy calculated from the temperature dependence of the binding constant did not match with the calorimetric enthalpy indicating conformational change in the protein upon surfactant binding. The surfactant binds to alpha-LA with one class of binding site, and the thermal unfolding results indicate it to be a stronger destabilizer than BSA. The fluorescence, circular dichroism, and differential scanning calorimetric results corroborate well with each other. The effect of ionic strength on the binding parameters suggests that TX-100 can bind to the protein surface via both hydrophobic and polar interactions depending upon the nature of the protein. The physical chemistry underlying the interactions between TX-100 and proteins has been presented. The mode of interaction of TX-100 with proteins is via direct binding, which has been discussed quantitatively in this work.     

The Photostabilization of Hemoglobin in Triton X-100 Aqueous Solution and Triton X-100/n-C5H11OH/H2O Microemulsion

The influence of UV-irradiation on the interaction of hemoglobin (Hb) with Triton X-100 is investigated by UV–Vis absorption spectroscopy, fluorescence spectroscopy and freeze-fractured transmission electron microscopy. It is found that in Triton X-100/H₂O systems Hb can convert to hemichrome but heme is not present, whereas in Triton X-100/n-C₅H₁₁OH/H₂O microemulsion Hb can convert to hemichrome and then induce the heme monomer to leave the hydrophobic cavity of Hb. UV-irradiation can also convert Hb to hemichrome, and subsequently make heme to be photodegraded, in which the conversion rate depends on the structure of the surfactant aggregates. Furthermore, in order to understand the mechanism of photostabilization of Hb in Triton X-100 systems, the photostabilization of heme in the Triton X-100 aqueous solutions and Triton X-100/n-C₅H₁₁OH/H₂O microemulsions has been studied.     

Influences of Triton X-100 micelle on the microstructure of HSA

The effects of Triton X-100 molecule and micelle on the microstructure and properties of HSA are studied by the some methods of UV spectrum, fluorescence spectrum, fluorescence polarization, circular dichroism, conductivity, and zeta potential. With the increase of Triton X-100 concentration, the UV absorbance, fluorescence intensity of HSA, and the system conductivity all first decrease and then increase. The zeta potential of HSA first goes up and then down. The percents of the β-sheet, random, turn structures, and the polarization of HSA increase but the percent of the α-Helix of HSA decreases. When Triton X-100 concentration is more than 1.0×10⁻³ mol l⁻¹, the structure parameters change obviously especially for the percents of random and turn structures.     

Probing mode and site of substrate water binding to the oxygen-evolving complex in the S2 state of photosystem II by 17O-HYSCORE spectroscopy

In the oxygen-evolving complex (OEC) of photosystem II (PSII) molecular oxygen is formed from two substrate water molecules that are ligated to a mu-oxo bridged cluster containing four Mn ions and one Ca ion (Mn4OxCa cluster; Ox symbolizes the unknown number of mu-oxo bridges; x >or= 5). There is a long-standing enigma as to when, where, and how the two substrate water molecules bind to the Mn4OxCa cluster during the cyclic water-splitting reaction, which involves five distinct redox intermediates (Si-states; i = 0,...,4). To address this question we employed hyperfine sublevel correlation (HYSCORE) spectroscopy on H217O-enriched PSII samples poised in the paramagnetic S2 state. This approach allowed us to resolve the magnetic interaction between one solvent exchangeable 17O that is directly ligated to one or more Mn ions of the Mn4OxCa cluster in the S2 state of PSII. Direct coordination of 17O to Mn is supported by the strong (A approximately 10 MHz) hyperfine coupling. Because these are properties expected from a substrate water molecule, this spectroscopic signature holds the potential for gaining long-sought information about the binding mode and site of one of the two substrate water molecules in the S2 state of PSII.     

Application of high-performance liquid chromatography to the purification of the putative intestinal peptide transporter

A membrane protein of relative molecular mass (Mr) 127,000 was identified by photoaffinity labelling as (a component of) the uptake system for small peptides and beta-lactam antibiotics in rabbit small intestine. This binding protein is a microheterogeneous glycosylated integral membrane protein which could be solubilized with non-ionic detergents and enriched by lectin affinity chromatography on wheat germ lectin agarose. For the final purification of this protein and separation from aminopeptidase N of Mr 127,000, fast protein liquid chromatography (FPLC) was used. Gel permeation, hydroxyapatite and hydrophobic interaction chromatography were not successful for the purification of the 127,000-dalton binding protein. By anion-exchange chromatography on a Mono Q column with either Triton X-100 or n-octylglucoside as detergent, a partial separation of the 127,000-dalton binding protein from aminopeptidase N was achieved. By cation-exchange chromatography on a Mono S HR 5/5 column at pH 4.5 using Triton X-100 as detergent also only a partial separation from aminopeptidase N could be achieved. If, however, Triton X-100 was replaced with n-octylglucoside, the binding protein for beta-lactam antibiotics and small peptides of Mr 127,000 could be completely separated from aminopeptidase N. These results indicate that Triton X-100 should be avoided for the purification of integral membrane proteins because mixed protein-detergent micelles of high molecular weight prevent a separation into the individual membrane proteins. The putative peptide transport protein was finally purified by rechromatography on Mono S and was obtained more than 95% pure as determined densitometrically after sodium dodecyl sulphate gel electrophoresis. By application of FPLC even microheterogeneous membrane glycoproteins from the intestinal mucosa can be purified to such an extent that a sequence analysis and immunohistochemical localization with antibodies prepared from the purified protein is possible.     

表面活性离子液体溴化N-十二烷基异喹啉与非离子表面活性剂Triton X-100在水溶液中的混合胶束

用等温滴定微量热法测定表面活性离子液体溴化N-十二烷基异喹啉([C₁₂iQuin]Br)与非离子表面活性剂Triton X-100混合物在水溶液中的临界胶束浓度。并以¹H核磁共振(NMR)和二维核Overhauser效应增强谱(2D NOESY)研究[C₁₂iQuin]Br与Triton X-100在混合胶束中的作用机理。研究结果显示：混合胶束中,Triton X-100分子的苯环定位于混合胶束的内核,聚氧乙烯链卷曲在异喹啉环周围。本文还应用规则溶液理论和浊点法对比研究了十二烷基三甲基溴化铵(DTAB)-Triton X-100混合胶束体系的相关性质。     

Surfactant-induced amorphous aggregation of tobacco mosaic virus coat protein: a physical methods approach

The interactions of non-ionic surfactant Triton X-100 and the coat protein of tobacco mosaic virus, which is an established model for both ordered and non-ordered protein aggregation, were studied using turbidimetry, differential scanning calorimetry, isothermal titration calorimetry, and dynamic light scattering. It was found that at the critical aggregation concentration (equal to critical micelle concentration) of 138 x 10(-6) M, Triton X-100 induces partial denaturation of tobacco mosaic virus coat protein molecules followed by protein amorphous aggregation. Protein aggregation has profound ionic strength dependence and proceeds due to hydrophobic sticking of surfactant-protein complexes (start aggregates) with initial radii of 46 nm. It has been suggested that the anionic surfactant sodium dodecyl sulfate forms mixed micelles with Triton X-100 and therefore reverses protein amorphous aggregation with release of protein molecules from the amorphous aggregates. A stoichiometric ratio of 5 was found for Triton X-100-sodium dodecyl sulfate interactions.     

ASSOCIATION OF POLAR LIPIDS TO SPINACH SUBCHLOROPLAST FRACTIONS EVOLVING OXYGEN

An O₂-evolving photosystem II (PSII) fraction was isolated from spinach chloroplasts using Triton X-100. The distribution of polar lipids is different from that in thylakoids: the ratio monogalactosyldiacylglycerol/digalactosyldiacylglycerol being higher and the level of sulfoquinovosyldiacylglycerol being lower in the PSII fraction. A large amount of phosphatidylglycerol containing trans -Δ₃-hexadecenoic remains associated to the PSII fraction. A possible role for molecules of phosphatidylglycerol containing trans -Δ₃-hexadecenoic acid in the regulation of energy transfer between the two photosystems is suggested.     

Mixed micellization of gemini surfactant with nonionic surfactant in aqueous media: a fluorometric study

Herein we report on the study of the interactions between alkanediyl-α,ω-type cationic dimeric (gemini) surfactant and the nonionic Triton X-100 in aqueous medium. The critical micelle concentrations of binary mixtures were determined by fluorometric study. Using the regular solution theory for the analysis of the experimental data, the attractive nature of interactions and synergistic behavior of gemini surfactant and Triton X-100 mixture were demonstrated. The micelle aggregation number was measured using steady state fluorescence quenching method. The micropolarity, binding constant and dielectric constant of mixed systems were determined from the ratio of peak’s intensity (I ₁/I ₃) in the pyrene fluorescence emission spectrum.