Tuberculosis associated haemophagocytic syndrome: two cases with a favourable outcome

Haemophagocytic syndrome is a heterogenous disease characterized by disordered macrophage activation associated with viral, bacterial or parasitic infection. The few reports of haemophagocytosis occurring in the presence of mycobacterial infection show a high mortality rate and we present two further cases notable for their favourable issue. Rapidity of diagnosis and immediate treatment could explain the avoidance of a fatal outcome.     

Beneficial Effects of Natural Mineral Waters on Intestinal Inflammation and the Mucosa-Associated Microbiota

Natural mineral water (NMWs) intake has been traditionally used in the treatment of various gastrointestinal diseases. We investigated the effect of two French NMWs, one a calcium and magnesium sulphate, sodium chloride, carbonic, and ferruginous water (NMW1), the other a mainly bicarbonate water (NMW2) on the prevention of intestinal inflammation. Intestinal epithelial cells stimulated with heat inactivated Escherichia coli or H₂O₂ were treated with NMWs to evaluate the anti-inflammatory effects. Moderate colitis was induced by 1% dextran sulfate sodium (DSS) in Balbc/J mice drinking NMW1, NWW2, or control water. General signs and histological features of colitis, fecal lipocalin-2 and pro-inflammatory KC cytokine levels, global mucosa-associated microbiota, were analyzed. We demonstrated that both NMW1 and NMW2 exhibited anti-inflammatory effects using intestinal cells. In induced-colitis mice, NMW1 was effective in dampening intestinal inflammation, with significant reductions in disease activity scores, fecal lipocalin-2 levels, pro-inflammatory KC cytokine release, and intestinal epithelial lesion sizes. Moreover, NMW1 was sufficient to prevent alterations in the mucosa-associated microbiota. These observations, through mechanisms involving modulation of the mucosa-associated microbiota, emphasize the need of investigation of the potential clinical efficiency of such NMWs to contribute, in human beings, to a state of low inflammation in inflammatory bowel disease.     

Consumption of Select Dietary Emulsifiers Exacerbates the Development of Spontaneous Intestinal Adenoma

Inflammation is a well-characterized critical driver of gastrointestinal cancers. Previous findings have shown that intestinal low-grade inflammation can be promoted by the consumption of select dietary emulsifiers, ubiquitous component of processed foods which alter the composition and function of the gut microbiota. Using a model of colitis-associated cancer, we previously reported that consumption of the dietary emulsifiers carboxymethylcellulose or polysorbate-80 exacerbated colonic tumor development. Here, we investigate the impact of dietary emulsifiers consumption on cancer initiation and progression in a genetical model of intestinal adenomas. In APC^min mice, we observed that dietary emulsifiers consumption enhanced small-intestine tumor development in a way that appeared to be independent of chronic intestinal inflammation but rather associated with emulsifiers’ impact on the proliferative status of the intestinal epithelium as well as on intestinal microbiota composition in both male and female mice. Overall, our findings further support the hypothesis that emulsifier consumption may be a new modifiable risk factor for colorectal cancer (CRC) and that alterations in host–microbiota interactions can favor gastrointestinal carcinogenesis in individuals with a genetical predisposition to such disorders.     

Mechanism of nickel-molybdenum alloy electrodeposition in citrate electrolytes

The kinetics of the induced codischarge of Mo with Ni in citrate-ammonia electrolytes was investigated by means of polarization and a.c. impedance measurements. Three potential ranges were considered. At low polarization, hydrogen evolution resulting from citrate reduction is the main reaction. The impedance plots exhibit a large capacitive loop with a small high frequency inflection characteristic of the development of a porous layer and a low frequency inductive feature. At intermediate polarization, the partial currents for Ni and Mo discharge increase in the same proportion; the hydrogen evolution is first constant and then rapidly decreases. Then a large low-frequency capacitive feature is observed on the impedance plots, whose size decreases with increasing polarization. At still higher polarization, the Mo discharge becomes increasingly controlled by diffusion which generates an additional capacitive loop. A reaction scheme is proposed which accounts for the polarization data and the major impedance features.     

Tracking a new cell-penetrating (W/R) nonapeptide, through an enzyme-stable mass spectrometry reporter tag

We have designed a mass stable reporter (msr) tag with m/z over 500, trifluoroacetyl(alpha,alpha-diethyl)Gly-Lys(Nepsilonbiotin)-(D)Lys-Cys, for the quantification of the uptake and study of the degradation processes of cell-penetrating peptides (CPP), by matrix assisted laser desorption/ionization time-of-flight (MALDI-TOF) mass spectrometry. This tag was found stable in cell lysis conditions. Using a quantitative MALDI-TOF mass spectrometry analysis based method, an accurate tracking of a new CPP and of its degradation products could be done. (1) The new msr(W/R) nonapeptide (H-RRWWRRWRR-NH2) enters chinese hamster ovary (CHO) K1 cells with a kinetic reaching a steady state after 30-60 min of incubation. This plateau was stable for 4 h and decreased slowly afterward. (2) The peptide msr(W/R) nonapeptide was not cytotoxic over 48 h incubation with CHO cells. (3) After 1 h incubation, the msr(W/R) nonapeptide accumulated with a 3-fold higher concentration than the extracellularly added concentration (7.5 microM). (4) The intracellular quantification was accurate with less than 3% of the quantified peptide being potentially membrane-bound. (5) There was no leakage of the full-length CPP outside the cells. And, finally, (6) analysis of the degradation process of this new CPP suggests that the peptide did not traffick to lysosomes.     

Preparation and properties of electroless Ni–Zn–P alloy films

Electroless deposition of Ni–Zn–P layers was studied on steel electrodes by varying the bath temperature (40–90°C), pH and chemical composition. The deposition parameters were optimized. Alloys containing 70–86 wt % Ni, 6–20 wt % Zn and 6–10 wt % P are obtained at 20 m h^–1 and 85°C. Corrosion measurements were performed in aerated 5% sodium chloride solution, the corrosion potential and current density are, respectively, –0.49 V/SCE and 2.6 A cm^–2.     

Determination of the antitumor agent depsipeptide in plasma by liquid chromatography on serial octadecyl stationary phases

We have cloned the rat fibroblast growth factor-2 (FGF-2) promoter region including 1058 base pairs (bp) of 5'-flanking DNA. Complete sequencing of this promoter region revealed a 74 bp domain between nucleotides-793 and-720 that was greater than 97% A/G-rich. A repeat of the sequence 5'-AGGGAGGG-3' separated by 11 bp was located at the core of this domain. A 37 bp A/G-rich oligonucleotide containing these AGGG-repeat sequences was synthesised, and tested for function on a minimal herpes simplex virus thymidine kinase (TK) promoter, fused to the firefly luciferase gene (TKp.luc), in transiently transfected neonatal rat cardiac myocytes. Promoter activity was stimulated approximately 3 fold in the presence of AGGG-repeat sequences. This effect was neither tissue or species-specific since TK promoter activity was increased approximately 11 fold in both rat and human glial tumor cells. Four specific complexes (Cl-4) were detected between neonatal rat heart nuclear proteins and the 37 bp A/G-rich oligonucleotide by gel mobility shift assay. Competition with excess unlabelled 37 bp A/G-rich oligonucleotide revealed that two complexes represented very high affinity/specificity interactions (C2 > C4) while Cl and C3 were of lower affinity. As a result, competition with up to a 25 fold molar excess of 37 bp A/G-rich oligonucleotide led to the loss of C2 and C4, and a corresponding and transient increase in the levels of Cl and C3, which themselves were reduced with more competitor oligonucleotide. The AGGG-repeat resembles the 5'-gGGGAGGG-3' sequence previously implicated in the response of the atrial natriuretic factor promoter to the alpha-adrenergic agonist, phenylephrine. Although an additional 1.5 fold increase in TK promoter activity was detected in the presence of the 37 bp A/G-rich oligonucleotide with phenylephrine treatment of transfected myocytes, this effect was not statistically significant. Furthermore, there was no difference in the gel mobility shift (Cl-4) pattern obtained with the 37 bp A/G-rich oligonucleotide and nuclear protein isolated from neonatal rat cardiac myocytes grown in the presence or absence of norepinephrine. These data suggest that the A/G rich sequences in the rat FGF-2 gene 5'-flanking DNA, including the AGGG-repeat, are able to confer stimulatory activity on a promoter in a tissue- and species-independent manner, but alone are not able to induce a significant phenylephrine response in neonatal rat cardiac myocytes.     

Electrodeposition of Ni-Cu-Mo ternary alloys from citrate electrolytes

Conditions for the electrodeposition of Ni–Cu–Mo alloys from citrate electrolytes have been developed. The composition variations of the deposits with electrolyte pH and concentration have been investigated. A maximum molybdenum and nickel content is obtained for a pH of 7 and for low copper and large citrate concentrations. Molybdenum and copper are preferentially discharged at low current density whereas at high current density nickel becomes predominant. The deposits have a nodular morphology similar to that of the binary Ni–Mo layers     

Kinetics of copper electrodeposition in citrate electrolytes

The kinetics of copper electrocrystallization in citrate electrolytes (0.5M CuSO₄, 0.01 to 2M sodium citrate) and citrate ammonia electrolytes (up to pH 10.5) were investigated. The addition of citrate strongly inhibits the copper reduction. For citrate concentrations ranging from 0.6 to 0.8 M, the impedance plots exhibit two separate capacitive features. The low frequency loop has a characteristic frequency which depends mainly on the electrode rotation speed. Its size increases with increasing current density or citrate concentration and decreases with increasing electrode rotation speed. A reaction path is proposed to account for the main features of the reduction kinetics (polarization curves, current dependence of the current efficiency and impedance plots) observed in the range 0.5 to 0.8 M citrate concentrations. This involves the reduction of cupric complex species into a compound that can be either included as a whole into the deposit or decomplexed to produce the metal deposit. The resulting excess free complexing ions at the interface would adsorb and inhibit the reduction of complexed species. With a charge transfer reaction occurring in two steps coupled by the soluble Cu(I) intermediate which is able to diffuse into the solution, this model can also account for the low current efficiencies observed in citrate ammonia electrolytes and their dependencies upon the current density and electrode rotation speed.Nomenclature b, b ₁, b ₁ ^* Tafel coefficients (V^–1) - bulk concentration of complexed species (mol cm^–3) - (si*) concentration of intermediate C^* atx=0 (mol cm^–3) - C concentration of (Cu Cit H)^2– atx=0 (mol cm^–3) - C C variation due to E - C concentration of complexing agent (Cit)^3- at the distancex (mol cm^–3) - C _o concentrationC atx=0 (mol cm^–3) - C _o C _o variation due to E - Cv _s bulk concentrationC (mol cm^–3) - (Cit H), (Cu), (Compl) molecular weights (g) - C _dl double layer capacitance (F cm^–2) - D diffusion coefficient of (Cit)^3- (cm²s^–1) - D ₁ diffusion coefficient of C^* (cm²s^–1) - E electrode potential (V) - f ₁ frequency in Equation 25 (s^–1) - F Faraday's constant (96 500 A smol^–1) - i, i ₁, i ₁ ^* current densities (A cm^–2) - i i variation due to E - Im(Z) imaginary part ofZ - j - k ₁, k ₁ ^* , K₁, K ₁ ^* , K₂, K rate constants (cms^–1) - K rate constant (s^–1) - K ₃ rate constant (cm³ A^–1s^–1) - R _t transfer resistance (cm²) - R _p polarization resistance (cm²) - Re(Z) real part ofZ - t time (s) - x distance from the electrode (cm) - Z _f faradaic impedance (cm²) - Z electrode impedance (cm²) Greek symbols maximal surface concentration of complexing species (molcm^–2) - thickness of Nernst diffusion layer (cm) - , ₁, ₂ current efficiencies - angular frequency (rads^–1) - electrode rotation speed (revmin^–1) - =K ^–1(s) - _d diffusion time constant (s) - electrode coverage by adsorbed complexing species - (in0) electrode coverage due toC _s - variation due to E     

Tachykinin peptides affect differently the second messenger pathways after binding to CHO-expressed human NK-1 receptors

The human NK-1 receptor transfected in Chinese hamster ovary (CHO) cells was studied with use of different tachykinin analogs: Substance P, [Pro9]SP, [Sar9, Met(O2)11]SP, [Gly9 psi (CH2CH2) Leu10]SP, Ac-Arg-septide, septide, [Gly9 psi (CH2CH2) Gly10]SP, NKA, [pGlu6]SP(6-11) and [Lys5]NKA(4-10). Binding experiments with [3H][Pro9]SP discriminated two classes of peptides with either high affinity (K iota in the nanomolar range) for the human NK-1 receptor or with low affinity (K iota in the micromolar range); this second group of peptides included NKA and [pGlu6]SP(6-11). In spite of these differences, both peptide families evoked potent stimulation of phosphatidylinositol hydrolysis (EC50 in the nanomolar range). In contrast, only NK-1 agonists, with high affinity, stimulated with great potency cyclic AMP formation (EC50 from 8 to 50 nM), whereas the second family of peptides were only weak agonists (EC50 in the micromolar range). RP 67580, CP 96345 and GR 94800, a NK-2 antagonist, were either competitive or uncompetitive inhibitors of inositol phosphates or cyclic AMP formations induced by [Pro9]SP, septide or NKA, independently of the agonist or the response studied. Thus, NKA, the presumed NK-2 endogenous peptide that may be co-released with SP, and the enzymatically produced C-terminal fragment of SP, [pGlu6]SP(6-11), may trigger specific pharmacological responses via the NK-1 receptor, at nanomolar concentrations, and thus regulate the action of SP at the NK-1 receptor.