表皮生长因子治疗兔角膜碱烧伤研究

本试验制成兔角膜碱烧伤模型,应用重组表皮生长因子（ｒｈＥＧＦ）滴眼剂对碱烧伤后的兔角膜溃疡创面进行治疗。６３只纯种新西兰白兔分为７组,每组９只,其中５组为治疗组,另２组为对照组,治疗组分别用每毫升０．５,５,２０,５０和１００μｇ表皮生长因子滴眼剂滴眼,对照组分别用纤维结合蛋白和氯霉素滴眼。伤后２４,４８,７２,９６及１２０ｈ裂隙灯荧光素染色,照像观察溃疡面积,经计算机图像处理,计算。结果显示５组治疗组创面愈合时间明显短于对照组,（Ｐ＜０．０５）。提示ＥＧＦ对角膜碱烧伤后的溃疡面愈合有促进作用。     

Reaction‐based probe for hydrogen sulfite: dual‐channel and good ratiometric response

We designed and synthesized a new series of intramolecular charge transfer (ICT) molecules (compounds T1, T2 and T3) by attaching various electron‐donating thiophene groups to the triphenylamine backbone with aldehyde group as the electron acceptor. Based on the nucleophilic addition reaction between hydrogen sulfite and aldehyde, all compounds could act as ratiometric optical probe for hydrogen sulfite and displayed efficient chromogenic and fluorogenic signaling. Upon the addition of hydrogen sulfite anions, probe T3 displayed apparent fluorescent color changes from yellowish‐green to blue, with a large emission wavelength shift (Δλ = 120 nm). T3 responded to hydrogen sulfite with high sensitivity and the detection limit was determined to be as low as 0.9 μM. At the same time, apparent changes in UV–vis spectra could also be observed. By virtue of the special nucleophilic addition reaction with aldehyde, T3 displayed high selectivity over other anions. Copyright © 2016 John Wiley & Sons, Ltd.     

Cell surface labeling of erythrocyte glycoproteins by galactose oxidase and Mn++-catalyzed coupling reaction with methionine sulfone hydrazide.

Methionine sulfone hydrazide (MSH) was coupled to 6-aldehydosugars and the reaction was found to be catalytically enhanced by Mn⁺⁺ ion under physiological condition. The reaction was applied to label surface glycoproteins of erythrocytes with [³⁵S]-MSH after treating cells with galactose oxidase. The slab gel electrophoretic pattern of surface glycoproteins in sodium dodecylsulfate-polyacrylamide can be printed on autoradiogram. At least ten glycoproteins of normal human erythrocytes were printed; five (c, d, e, g, and k) were major bands, and of these four (c, d, e, and g) corresponded to “PAS I, II′, II, and III”. Others are hitherto unrecognized. Two intense bands each corresponds to c, and g, and two new bands, d′ and e′, were printed in desialylated fetal erythrocytes; intact fetal erythrocytes did not show significant label.     

A method for chromatographic separation and fluorometric quantification of 2'',3''-cyclic nucleotide-3''-phosphodiesterase reaction products

Treatment of hydrochloric acid with sodium sulfite prior to the acid hydrolysis of bovine pancreatic ribonuclease A has been found to suppress the oxidation of cystine, methionine, and tyrosine without adversely affecting the recoveries of other amino acids. Statistical analysis of the results indicated that the assumption of the independence of the mean and the variance, an assumption commonly used in the evaluation of the effects of various treatments, may not be valid in evaluating antioxidants used in the acid hydrolysis of proteins.     

Transformation and movement of zinc in an alkali soil and their influence on the yield and uptake of zinc by rice and wheat crops

Summary In the summer of 1980, a field experiment was started to evaluate the direct and residual effect of applied zinc (as zinc sulphate) on the yield and chemical composition of rice and wheat grown as crops in sequence, on an alkali soil. The treatments comprised six rates of zinc 0, 2.25, 4.5, 9.0, 18.0 and 27.0 kg ha⁻¹ applied either only once to the first crop, or repeated to each successive crop in a split plot design with 4 replications. Gypsum at 14 t ha⁻¹, was applied uniformly to all plots. The results show that with respect to increase of yield and available zinc content of soil, an application of 2.25 kg ha⁻¹ zinc frequently to each crop was better than a single high dose. A major portion of the applied zinc accumulated in the 0 to 10 cm soil layer; the movement of zinc to lower layers was negligible. Zinc applications increased the concentration of exchangeable < complexed < amorphous sesquixoides-bound zinc > crystalline sesquioxide-bound zinc fractions. Amorphous sesquixoides bound the major portion of the applied zinc compared to other fractions. Exchangeable and amorphous sesquioxide-bound zinc fractions contributed significantly more to zinc uptake by rice, than the other fractions. DTPA extracted zinc more readily from exchangeable and complexed fractions than from sesquioxides. Application of zinc increased the DTPA extractable zinc and hence zinc uptake by plants.     

Comparison of the diversity of sulfate-reducing bacterial communities in the water column and the surface sediments of a Japanese meromictic lake

The diversity and abundance of sulfate-reducing bacteria (SRB) were investigated in Lake Suigetsu, a meromictic lake in Japan characterized by a permanent oxycline at a depth between 3 and 8 m separating the aerobic freshwater epilimnion from the anaerobic, saline, sulfidogenic hypolimnion. A quantitative competitive PCR targeting the gene coding for a portion of the α-subunit of dissimilatory sulfite reductase (dsrA) was used to assess the distribution of the SRB in the stratified water column and the surface sediments. The diversity of the SRB communities was assessed using a sequence analysis of the differing dsrA isomers. The dsrA gene copy numbers of SRB in the hypolimnic waters were from 9.6 × 10³ to 7.5 × 10⁵ copies ml⁻¹, whereas higher dsrA copy numbers of SRB were observed in surface sediments, ranging from 1.8–8.1 × 10⁷ copies ml⁻¹ as estimated by competitive PCR. Phylogenetic analysis of the dsrA sequences retrieved from the surface sediments shows most belong to a deeply branching lineage of diverse dsrA sequences not related to any cultured SRB group. In contrast, dsrA sequences found in the oxycline waters were related to sequences of members of the genera Desulfonema, Desulfosarcina, and Dusulfococcus and to sequences of the incomplete oxidizers from the Desulfobulbaceae family. Diversity and abundance of dsrA genes significantly differed between the samples from the oxycline waters and the surface sediments of Lake Suigetsu, indicating habitat-specific SRB communities may contribute to the biogeochemical cycling of carbon and sulfur.     

High genetic similarity between two geographically distinct strains of the sulfur-oxidizing symbiont 'Candidatus Thiobios zoothamnicoli'

The giant marine ciliate Zoothamnium niveum ( Ciliophora, Oligohymenophora ) is obligatorily covered by a monolayer of putative chemoautotrophic sulfur-oxidizing (thiotrophic) bacteria. For Z. niveum specimens from the Caribbean Sea it has been demonstrated that this ectosymbiotic population consists of only a single pleomorphic phylotype described as Candidatus Thiobios zoothamnicoli. The goal of our study was to identify and phylogenetically analyse the ectosymbiont(s) of a recently discovered Z. niveum population from the Mediterranean Sea, and to compare marker genes encoding key enzymes of the carbon and sulfur metabolism between the two symbiont populations. We identified a single bacterial phylotype representing the ectosymbiont of Z. niveum from the Mediterranean population showing 99.7% 16S rRNA gene (99.2% intergenic spacer region) similarity to the Caribbean Z. niveum ectosymbiont. Genes encoding enzymes typical for an inorganic carbon metabolism [ribulose 1,5-bisphosphate carboxylase/oxygenase (RuBisCO)] and for sulfur metabolism (5'-adenylylsulfate reductase, dissimilatory sulfite reductase) were detected in both symbiotic populations. The very high amino acid sequence identity (97–100%) and the high nucleic acid sequence identity (90–98%) of these marker enzymes in two geographically distant symbiont populations suggests that the association of Z. niveum with Cand . Thiobios zoothamnicoli is very specific as well as temporally and spatially stable.     

Could a strong alkali deproteinization replace the standard lysis step in alkaline single cell gel electrophoresis (comet) assay (pH > 13)?

The alkaline version of single cell gel electrophoresis (comet) assay is widely used for evaluating DNA damage at the individual cell level. The standard alkaline method of the comet assay involves deproteinization of cells embedded in agarose gel using a high salt–detergent lysis buffer, followed by denaturation of DNA and electrophoresis using a strong alkali at pH > 13 [N.P. Singh, M.T. McCoy, R.R. Tice, E.L. Schneider, A simple technique for quantitation of low levels of DNA damage in individual cells, Exp. Cell. Res. 175 (1988) 184–191]. However, a recent report showed that a strong alkali treatment results in simultaneous deproteinization of cells and denaturation of genomic DNA [P. Sestili, C. Martinelli, V. Stocchi, The fast halo assay: an improved method to quantify genomic DNA strand breakage at the single cell-level, Mutat. Res. 607 (2006) 205–214]. This study was carried out to test whether the strong alkali deproteinization of cells could replace the high salt–detergent lysis step used in the standard method of the alkaline comet assay. Peripheral blood lymphocytes from 3 healthy individuals were irradiated with gamma rays at doses varying between 0 and 10 Gy. Following irradiation, the comet assay was performed according to the standard alkaline method (pH > 13) and a modified method. In the modified method, agarose embedded cells were treated with a strong alkali (0.3 M NaOH, 0.02 M Trizma and 1 mM EDTA, pH > 13) for 20 min to allow deproteinization of cells and denaturation of DNA. This was followed by electrophoresis using the same alkali solution to obtain comets. DNA damage expressed in terms of comet tail length, percentage of DNA in comet tail and tail moment obtained by the standard alkaline method and the modified method were compared. In both methods, DNA damage showed a good correlation with the dose of gamma ray. The results indicate a satisfactory sensitivity of the modified method in detecting radiation-induced DNA damage in human peripheral blood lymphocytes.     

Solid-state 23Na NMR determination of the number and coordination of sodium cations bound to Oxytricha nova telomere repeat d(G4T4G4)

We report a solid-state (23)Na NMR study of the bound sodium cations in a G-quadruplex formed by Oxytricha nova telomere DNA repeat, d(G(4)T(4)G(4)) (Oxy-1.5). Using a 2D multiple-quantum magic-angle spinning (23)Na NMR method, we observed three sodium cations residing inside the quadruplex channel of the Na(+) form of Oxy-1.5. Each of these sodium cations is sandwiched between two G-quartets. We found no evidence for sodium cations in the T(4) loop region. For comparison, solid-state (15)N MAS NMR spectra were also obtained for the (15)NH(4)(+) form of Oxy-1.5. The insufficient resolution in the (15)N MAS NMR spectra did not permit determination of the number of NH(4)(+) ions inside the quadruplex channel. The solid-state (23)Na and (15)N NMR spectra for Oxy-1.5 were also compared with those obtained for guanosine 5'-monophosphate.