Biostimulation of Na,K-ATPase by low-energy laser irradiation (685 nm, 35 mW): comparative effects in membrane, solubilized and DPPC:DPPE-liposome reconstituted enzyme

OBJECTIVE: The aim of the present work was to investigate the effect of low-energy laser irradiation (685 nm, 35 mW) on the ATPase activity of the different forms of the Na,K-ATPase. METHODS: Membrane-bound and solubilized (alphabeta)(2) form of Na,K-ATPase was obtained from the dark red outer medulla of the kidney and proteoliposomes of DPPC:DPPE and Na,K-ATPase was prepared by the co-solubilization method. Irradiations were carried out at 685 nm using an InGaAIP diode laser. RESULTS: The ATPase activity of the membrane fraction was not altered with exposition to irradiation doses between 4 and 24 J/cm(2). However, with irradiation doses ranging from 32 to 40 J/cm(2), a 28% increase on the ATPase activity was observed while when using up to 50 J/cm(2) no additional enhancement was observed. When biostimulation was done using the solubilized and purified enzyme or the DPPC:DPPE-liposome reconstituted enzyme, an increase of about 36-40% on the ATPase activity was observed using only 4-8 J/cm(2). With irradiation above these values (24 J/cm(2)) no additional increase in the activity was observed. These studies revealed that the biostimulation of ATPase activity from different forms of the Na,K-ATPase is dose dependent in different ranges of irradiation exposure. The stimulation promoted by visible laser doses was modulated and the process was reverted after 2 h for the enzyme present in the membrane and after about 5 h for the solubilized or the reconstituted in DPPC:DPPE-liposomes.     

Claisen rearrangement induced by low-energy collision of ESI-generated, protonated benzyloxy indoles

The Claisen rearrangement is a well-known process occurring in condensed phase. In the gas-phase protonated allyl phenyl ethers, propargyl phenyl ethers, and N-allyl aniline produced by positive ion chemical ionization undergo Claisen rearrangement. This reaction has been observed even in the case of odd-electron molecular ions. Phenyl allenyl ether molecular ions actually undergo Claisen rearrangement, producing intense [M - CO](+*) ions. In this investigation, the behavior of protonated benzyloxy indole and some of its derivatives, obtained in electrospray conditions, is described. Low-energy MS/MS experiments carried out on [M + H](+) species show CO loss and an unexpected water loss: both can be justified only by the occurrence of Claisen rearrangement. Deuterium labeling experiments confirm this mechanism. The influence of different substituents in the indole moiety is discussed.     

An investigation on the nature of the peptide at m/z 904, overexpressed in plasma of patients with colorectal cancer and familial adenomatous polyposis

In an investigation devoted to the search for plasma markers for colorectal cancer (CRC), carried out by matrix-assisted laser desorption/ionization (MALDI) mass spectrometry, a series of overexpressed peptides were identified in the plasma of patients. Among them the peptide with molecular weight 903 Da was the most abundant one, with a mean +/- (SD) relative abundance of 37 +/- 17% and a frequency over 60%. Interestingly, also in plasma samples of ten subjects affected by familial adenomatous polyposis (FAP), the peptide with molecular weight 903 was overexpressed. In this investigation, MALDI/MS/MS experiments were carried out on the ion at m/z 904 detected in the MALDI mass spectra of CRC and FAP patients. The data analysis by SwissProt.2007.01.09 indicates that this peptide is due to the sequence RPPGFSPF, found in the kininogen-1 precursor, which is an alpha-2-thiol proteinase inhibitor. In the case of subjects affected by a particular FAP syndrome, the MALDI/MS/MS spectra were quite different from those obtained from CRC and FAP patients. In fact, two sequences have been evidenced: RPPGFSPF belonging to kininogen-1 precursor, and PRKSSSSR belonging to Forkhead box protein 01A.     

DNA and RNA noncovalent interaction of platinum(II) polypyridine complexes

A comparative investigation of the noncovalent interaction of the platinum(II) polypyridine complexes [Pt(dipy)(n-Rpy)2]2+ and [Pt(4,4'-Me2dipy)(2-Rpy)2]2+ (dipy = 2,2'-dipyridine; Me = CH3; n = 2-4; R = H or CH3) with double-helical DNA (calf thymus) and RNA [poly(A).poly(U)] has been conducted. With the exception of [Pt(dipy)(2-Mepy)2]2+, all of the complexes interact strongly, by intercalation, with both nucleic acids giving rise to large changes in the electronic spectra and induced circular dichroism signals; in addition, viscosity experiments on rodlike DNA and RNA show that both biopolymers elongate upon interaction with the complexes. The binding constant values, KB, determined at 25 degrees C, indicate that, at 0.101 M ionic strength, the affinity for poly(A).poly(U) is strongly dependent on the complexes nature, while for DNA it is leveled off. [Pt(dipy)(2-Mepy)2]2+ binds to DNA but does not interact appreciably with poly(A).poly(U).     

Dissociative double photoionization of N2 using synchrotron radiation: appearance energy of the N2+ dication

Photoionization cross sections for the production of the doubly charged ion N2+ from N2 have been measured by means of synchrotron radiation in the photon energy range from 50 to 110 eV. The appearance energy for N2+ has been determined as 55.2+/-0.2 eV, i.e., about 1.3 eV higher than the spectroscopic dissociation limit leading to the charge asymmetric dissociation channel N2+(2P)+N(4S) at 53.9 eV. The onset of a second threshold at 59.9+/-0.2 eV is detected and the energy dependence of photoion intensities near the threshold regions is interpreted in terms of the Wannier theory. The production of the N2+ dication is discussed in terms of direct and indirect mechanisms for dissociative charge asymmetric photoionization and by comparison with the potential energy curves of the intermediate N(2)2+ dication. Experimental evidences for the opening of the Coulomb explosion channel N2++N+ at high photon energies are provided by measuring the kinetic energy release spectra of N2+ fragments at selected photon energies.     

Pre-equilibrium γ ray emission in different reaction mechanisms at 8 MeV/nucleon

Recent experimental results on particles-γ coincidence measurements on the systems ¹²C +⁶⁴Ni and ³⁵Cl +⁶⁴Ni at about 8 MeV/nucleon are interpreted as due to the effect of a Dipole pre-equilibrium emission produced during the damping of the proton-neutron relative collective motion in very deformed intermediate systems formed in the first instants of the collision. The pre-equilibrium effects are evaluated through semiclassic kinetic theories and through modified statistical approach to include non-stationary effects in Fusion processes, Massive Transfer reactions (in the ¹²C +⁶⁴Ni system) and in Binary Dissipative reactions (in the ³⁵Cl +⁶⁴Ni system). In particular the study performed on the dipole molecular component allows to establish a link between the above phenomenon and the charge and mass transfer process in quasi-peripheral reactions. Received: 15 April 1998 / Revised version: 8 June 1998     

Interferometric focal length measurement of power-distributed lenses

An interferometric method for measuring the focal length of power-distributed lenses is described. The test lens is illuminated by a regular pitch interferometric pattern produced by a reflective diffraction grating interferometer. In order to measure the focal length, a CCD camera digitizes the image of the pattern magnified by the lens, and fast Fourier transformed to reconstruct the phase modulo 2π along each row. The change in spatial frequency is determined by unwrapping the phase along each row of the digitized imaged pattern. The technique is used for measuring the focal length distribution inside the progression corridor of both positive and negative progressive lenses.     

Renormalization of non-semisimple gauge models with the background field method

We study the renormalization of non-semisimple gauge models quantized in the 't Hooft-background gauge to all orders. We analyze the normalization conditions for masses and couplings compatible with the Slavnov-Taylor and Ward-Takahashi Identities and with the IR constraints. We take into account both the problem of renormalization of CKM matrix elements and the problem of CP violation and we show that the Background Field Method (BFM) provides proper normalization conditions for fermion, scalar and gauge field mixings. We discuss the hard and the soft anomalies of the Slavnov-Taylor Identities and the conditions under which they are absent.     

Cooperative stabilisation of 14-3-3σ protein–protein interactions via covalent protein modification

14-3-3 proteins are an important family of hub proteins that play important roles in many cellular processes via a large network of interactions with partner proteins. Many of these protein–protein interactions (PPI) are implicated in human diseases such as cancer and neurodegeneration. The stabilisation of selected 14-3-3 PPIs using drug-like ‘molecular glues’ is a novel therapeutic strategy with high potential. However, the examples reported to date have a number of drawbacks in terms of selectivity and potency. Here, we report that WR-1065, the active species of the approved drug amifostine, covalently modifies 14-3-3σ at an isoform-unique cysteine residue, Cys38. This modification leads to isoform-specific stabilisation of two 14-3-3σ PPIs in a manner that is cooperative with a well characterised molecular glue, fusicoccin A. Our findings reveal a novel stabilisation mechanism for 14-3-3σ, an isoform with particular involvement in cancer pathways. This mechanism can be exploited to harness the enhanced potency conveyed by covalent drug molecules and dual ligand cooperativity. This is demonstrated in two cancer cell lines whereby the cooperative behaviour of fusicoccin A and WR-1065 leads to enhanced efficacy for inducing cell death and attenuating cell growth.

The aminothiol WR-1065 covalently modifies 14-3-3σ to stabilse its interactions with p53 and ERα. It enhances the effect of fusicoccin A via a cooperative mechanism that leads to 14-3-3 partner-protein specific activty against cancer cells.