Expression of a Chitinase Gene from <Emphasis Type="Italic">Metarhizium anisopliae</Emphasis> in Tobacco Plants Confers Resistance against <Emphasis Type="Italic">Rhizoctonia solani</Emphasis>

The chit1 gene from the entomopathogenic fungus Metarhizium anisopliae, encoding the endochitinase CHIT42, was placed under the control of the CaMV 35S promoter, and the resulting construct was transferred to tobacco. Seventeen kanamycin-resistant transgenic lines were recovered, and the presence of the transgene was confirmed by polymerase chain reactions and Southern blot hybridization. The number of chit1 copies was determined to be varying from one to four. Copy number had observable effects neither on plant growth nor development. Substantial heterogeneity concerning production of the recombinant chitinase, and both general and specific chitinolytic activities were detected in leaf extracts from primary transformants. The highest chitinase activities were found in plants harboring two copies of chit1 inserts at different loci. Progeny derived from self-pollination of the primary transgenics revealed a stable inheritance pattern, with transgene segregation following a mendelian dihybrid ratio. Two selected plants expressing high levels of CHIT42 were consistently resistant to the soilborne pathogen Rhizoctonia solani, suggesting a direct relationship between enzyme activity and reduction of foliar area affected by fungal lesions. To date, this is the first report of resistance to fungal attack in plants mediated by a recombinant chitinase from an entomopathogenic and acaricide fungus.     

Thermal properties of anhydride-cured bio-based epoxy blends

Epoxidized palm oil (EPO) (0–12 wt%) was added into petrochemical-based epoxy blends (diglycidyl ether of bisphenol-A (DGEBA)/cycloaliphatic epoxide resin/epoxy novolac resin) to develop a thermal curable bio-based epoxy system. The thermal behaviors of the EPO, epoxy blends (EB), and bio-based epoxy blends (EB/EPO) were characterized using differential scanning calorimetry (DSC), dynamic mechanical thermal analysis (DMT) and thermo-mechanical analysis (TM). The glass transition temperature (T _g) and storage modulus (E′) of the EB/EPO system was reduced with the increasing of the EPO loading. This is attributed to the plasticizing effect of the EPO. It was found that epoxy blends with higher loading of EPO possessed higher coefficient of thermal expansion (CTE) and tanδ value. This is due to the increase of the free volume and chain flexibility in the three-dimensional network of the epoxy blends. The internal thermal stresses of the EB/EPO were decreased as the increasing loading of EPO, owing to the reduction of crosslink density, modulus of elasticity, and T _g in the epoxy blends.     

Enhanced expression of B-subunit of Escherichia coli heat-labile enterotoxin in tobacco by optimization of coding sequence

Escherichia coli heat-labile toxin (LT) is a potent mucosal immunogen and immunoadjuvant for coadministered antigens. We synthesized a gene encoding the B-subunit of LT(LTB) adapted to the coding sequence of tobacco plants and fused to the endoplasmic reticulum retention signal SEKDEL to enhance its level of expression in plants. The synthetic LTB gene was cloned into a plant expression vector adjacent to the CaMV 35S promoter and was introduced into tobacco by Agrobacterium-mediated transformation. The amount of LTB protein detected in transgenic tobacco leaves was 2.2% of the total soluble plant protein, which is approx 200-fold higher than in previous reports of native LTB gene expression in transgenic plants. Enzyme-linked immunosorbent assay indicated that plant-synthesized LTB protein bound specifically to G_M1-ganglioside, suggesting that the LTB subunits formed active pentamers.     

Generation of a Recombinant Full-Length Human Antibody Binding to Botulinum Neurotoxin A

In order to develop a recombinant full-length human anti-botulinum neurotoxin A (BoNT/A) antibody, human peripheral blood mononuclear cells (PBMC) were collected from three healthy volunteers and induced for BoNT/A-specific immune response by in vitro immunization. The genes encoding human Fd fragment, consisting of antibody heavy chain variable region and constant region 1 with the genes encoding antibody light chain, were cloned from the immunized PBMC. Afterwards, one combinatory human antigen-binding fragment (Fab) library was constructed using a lambda phage vector system. The size of the constructed library was approximately 10⁵ Escherichia coli transformants. After screening the library by BoNT/A antigen using a plaque lifting with immunostaining approach, 55 clones were identified as positive. The Fab gene of the most reactive clone exhibiting particularly strong BoNT/A binding signal was further subcloned into a full-length human IgG1 antibody gene template in an adenoviral expression vector, in which the heavy and light chains were linked by a foot-and-mouth-disease virus-derived 2A self-cleavage peptide under a single promoter. After the full-length human IgG1 was expressed in mammalian cells and purified with protein L column, sodium dodecyl sulfate-polyacrylamide gel electrophoresis showed that the heavy and light chains of the antibody were cleaved completely. The affinity expressed as the dissociation constant (K _d) for the recombinant human antibody to bind to BoNT/A was determined by indirect enzyme-linked immunosorbent assay and results confirmed that the recombinant full-length human antibody retained BoNT/A-binding specificity with K _d value of 10⁻⁷ M.     

High Levels of Expression of Fibroblast Growth Factor 21 in Transgenic Tobacco (<Emphasis Type="Italic">Nicotiana benthamiana)</Emphasis>

Fibroblast growth factor-21 (FGF21) is a hepatic hormone that plays a critical role in metabolism, stimulating fatty acid oxidation in the liver and glucose uptake in adipose tissue. In this study, we produced tobacco plants expressing human recombinant FGF21 (hFGF21) via Agrobacterium-mediated transformation using a potato virus X (PVX)-based vector (pgR107). The vector contained the sequence encoding the human FGF21 gene fused with green florescence protein and a histidine tag. The recombinant plasmid was introduced into leaf cells of Nicotiana benthamiana (a wild Australian tobacco) via Agrobacterium-mediated agroinfiltration. As determined by fluorescence and Western blot of leaf extracts, the hFGF21 gene was correctly translated in tobacco plants. Seven days after agroinfection, the recombinant hFGF21 had accumulated to levels as high as 450 μg g⁻¹ fresh weight in leaves of agroinfected plants. The recombinant hFGF21 was purified from plant tissues by Ni–NTA affinity chromatography, and the purified hFGF21 stimulated glucose uptake in 3T3/L1 cells. This indicated that the recombinant hFGF21 expressed via the PVX viral vector in N. benthamiana was biologically active.     

Carrageenan as an elicitor of induced secondary metabolites and its effects on various growth characters of chickpea and maize plants

The effects of polysaccharide elicitor k-carrageenan obtained from Hypnea musciformis, red algae on the production of Induced Secondary Metabolites, ISMs (the disease resistance compounds) and on various growth characters of chickpea and maize plants were studied. Experiments were conducted in the field of PCSIR Laboratories Complex Karachi during December 2008–April 2009 in randomized complete block design with three replications. Three elicitor treatments were used, a solid preparation in which the elicitor was mixed with soil (T₂ 1 mg/g) and applied around the seeds in the soil. The two other preparations were liquid, T₁ and T₃ at a concentration of 100 μg glc eq ml⁻¹ and were applied around the sowing seeds and as a foliar spray on the plants, respectively. Statistical analysis of the data revealed that these treatments significantly enhanced all the growth characters of chickpea except T₂ that gave the nonsignificant difference in the plant height. Maximum plant height (80.3 cm), number of pods plant⁻¹ (76.2), number of branches plant⁻¹ (25.0), number of leaves plant⁻¹ (125.6), earlier flowering and high ISMs contents in leaves, stem and grains of chickpea were recorded in T₁ treated chickpea plants. In maize plants only T₁ and T₃ treatments (with minor exceptions) had significant effects on few characters like plant height, stem diameter, number of leaves plant⁻¹ and on ISMs contents in leaves while number of cobs plant⁻¹ and flowering time were nonsignificantly affected by these treatments. These results suggested that k-carrageenan elicitor can be used as a potent plant protectant as well as growth promoting agent especially for chickpea plants.     

Comparison of the fragility index of different eudragit polymers determined by activation enthalpies

The present study aimed to apply fragility index (m) of polymers in the determination of the optimal amount of plasticizer in polymer films. The fragility index of different Eudragit polymers (RS, RL, EPO) was assessed by differential scanning calorimerty (DSC), applying the Arrhenius connection (logq–1/T _g). The fragility of Eudragit EPO films proved to be the highest, while in the case of RS and RL, the increase of the alkyl-chain length caused the increase of fragility. Studying the effect of plasticizer (triethyl citrate, TEC) on the m value of Eudragit RL and RS films, a near linear reduction of the fragility index could be observed between 5–30% TEC concentration, but above 30%, this value leveled out to constant.     

Transgenic Expression and Functional Characterization of Human Platelet Derived Growth Factor BB (hPDGF-BB) in Tobacco (Nicotiana tabacum L.)

Recombinant human platelet derived growth factor BB (rhPDGF-BB) is clinically approved for treating diabetic neuropathic ulcers. Plant-based expression systems offer less expensive ways of producing recombinant drugs, which do not require purification for clinical use. From this perspective, rhPDGF-BB is an ideal candidate for expression in plants as it can be applied topically. Here, we report a proof of concept study, in which rhPDGF-BB was expressed in tobacco plants, and its biological activity was tested in vitro. The mature human platelet derived growth factor BB (hPDGF-BB) gene was codon-optimized for tobacco and fused with ER targeting and retention signals, 5′ and 3′ UTRs of arc5-1 gene along with CaMV 35S promoter, and then, transferred by Agrobacterium-mediated transformation. Gene and protein expression of hPDGF-BB were confirmed by PCR and immunoblot studies. Bioactivity of hPDGF-BB expressed protein was determined by in vitro assays such as proliferation and migration in NIH3T3 cells. Our data reveals that total soluble proteins containing hPDGF-BB from transgenic plants showed a 4.5-fold increase in fibroblast proliferation compared to non-transgenic plants. Furthermore, plant-made rhPDGF-BB induced chemotaxis of treated cells and promoted wound healing in vitro. These results clearly demonstrate that functionally active rhPDGF-BB protein can be produced in plants and might have therapeutic benefits.     

Isolation and characterization of an anti-recombinant erythropoietin single-chain antibody fragment using a phage display antibody library

The production of a large amount of specific antibodies against erythropoietin (EPO) is necessary for both clinical treatment and doping control. However, the weak immunogenicity of EPO and the side effects of excessive injection make the conventional immunological protocol rather inefficient and time-consuming. In this study, a single-chain antibody fragment of variable region (scFv) against recombinant human erythropoietin (rHuEPO) was produced after three rounds of panning a phage display antibody library. The selected scFv-B₂ was expressed in soluble form in Escherichia coli DH5α F′ and purified by His-bond nickel affinity chromatography with a yield of about 1–2 mg of antibody in 1 L of the culture supernatant. The molecular weight of the scFv was estimated to be 29 kDa by sodium dodecyl sulfate polyacrylamide gel electrophoresis and the affinity constant was found to be 1.0×10⁸ L mol⁻¹ based on a competitive indirect enzyme-linked immunosorbent assay (CI-ELISA). The potential ability of the scFvs for immunopurification of rHuEPO from related sample was demonstrated by using a double-antibody sandwich ELISA. The reported method is a very powerful tool to produce specific antibodies for rHuEPO detection demands.     

Molecular Structure and Conformations of Chloral (CCl3CHO) in the Ground and Lowest Triplet States

This paper reports on an ab initio quantum mechanical calculation of the structure of the conformationally nonrigid chloral (CCl₃CHO) molecule in the ground (S₀) and lowest excited triplet (T₁) states. Electronic excitation causes substantial changes in molecular geometry: the CCl₃ top is rotated, and the carbonyl (CCHO) fragment becomes nonplanar. For the torsional (S₀ and T₁) and inversion (T₁) nuclear vibrations, one- (S₀ and T₁) and two-dimensional (T₁) vibrational problems are solved; a relationship is found between the torsional and inversion vibrations in the T₁ state. The results are compared with the data of analogous calculations for the acetaldehyde molecule in the T₁ state.     

细胞内不同形态Gd基MRI造影剂的T1/T2弛豫性能及造影效果

将具有良好生物膜穿透性的异烟肼(INH)和Gd-DO3A偶联,合成了小分子MRI造影剂Gd-DO3A-INH;利用脉冲电转染技术标记间充质干细胞,有效提高了进入细胞的Gd-DO3A-INH浓度,并诱导部分游离态Gd-DO3A-INH在细胞质中自组装成纳米粒子。细胞样品的TEM观察到细胞内形成了Gd-DO3A-INH纳米粒子;细胞传代实验和体外MRI揭示了2种不同状态的Gd-DO3A-INH对细胞水质子弛豫速率的影响机制,以及细胞传代过程中细胞内2种不同状态Gd-DO3A-INH的浓度涨落引起的MRI造影效果的变化机制。     

Characterization of binding affinities in a chromatographic system by suspended state HR/MAS NMR spectroscopy

In the current work a racemate of (R)‐ and (S)‐benzylmandelate was separated with a stereoselective polysaccharide‐based chiral stationary phase by HPLC. To elucidate the occurring chiral molecular recognition processes in the heterogeneous system used, NMR spectroscopy was chosen under high resolution/magic angle spinning (HR/MAS) NMR conditions in the suspended state. Therefore, and as a proof of concept, a combination of several NMR methods such as spin–lattice relaxation time (T₁) measurements (T₁), the saturation transfer difference, and the 2D experiment of the transferred nuclear overhauser enhancement spectroscopy technique were applied. With HR/MAS NMR it is feasible to combine NMR and chromatography to achieve further insights into the separation process. Copyright © 2009 John Wiley & Sons, Ltd.     

Ab initio study of the structure and conformations of 2-fluoroethanal in the ground and lowest excited electronic states

The structure of the conformationally flexible 2-fluoroethanal molecule (CH₂FCHO, FE) in the ground (S₀) and lowest excited triplet (T₁) and singlet (S₁) electronic states was investigated by ab initio quantum-chemical methods. The FE molecule in the S₀ state was found to exist as two conformers, viz., as cis (the F—C—C—O angle is 0°) and trans (the F—C—C—O angle is 180°) conformers. On going both to the T₁ and S₁ states, the FE molecule undergoes substantial structural changes, in particular, the CH₂F top is rotated with respect to the core and the carbonyl CCHO fragment becomes nonplanar. The potential energy surfaces for the T₁ and S₁ states are qualitatively similar, viz., six minima in each of the excited states of FE correspond to three pairs of mirror-symmetrical conformers. Based on the potential energy surfaces calculated for the FE molecule in the T₁ and S₁ states, the one-dimensional problems on the torsion and inversion nuclear motions as well as the two-dimensional torsion-inversion problems were solved.     

Transgenic Tobacco Expressing <Emphasis Type="Italic">Zephyranthes grandiflora</Emphasis> Agglutinin Confers Enhanced Resistance to Aphids

Plant lectins have been reported as transgenic resistance factors against a variety of insect pests. Herein, homologous analysis demonstrated that Zephyranthes grandiflora agglutinin (ZGA) exhibited high similarity with other monocot mannose-binding lectins (MBLs). Phylogenetic analysis revealed that it had taxonomical relationships with insecticidal MBLs. Subsequently, a plasmid expression vector pBI121 containing zga gene (pBIZGA) was constructed using the zga sequence, under the control of CaMV35S promoter and nos terminator. pBIZGA was then integrated into the genome of Nicotiana tabacum L. Polymerase chain reaction and Southern blot analysis demonstrated that this zga gene was integrated into the plant genome. Western blotting and agglutinating activity analysis also showed that transgenic tobacco plants expressed different levels of ZGA. Carbohydrate inhibition analysis indicated that recombinant ZGA and the native shared the same carbohydrate-binding specificity. Moreover, genetic analysis confirmed Mendelian segregation (3:1) of the transgenic in T1 progenies. In planta bioassays on T0 plants and their progenies indicated that expressed ZGA had an effect on reducing the survivability and fecundity of tobacco aphids (Myzus nicotianae). These findings demonstrate that the novel zga gene of ZGA can be expressed in crop plants susceptible to various sap-sucking insects.     

Triplet excited states of nitronaphthalenes. IV. 1,2- and 1,8-dinitronaphthalenes

Nanosecond flash photolysis of 1,2- and 1,8-dinitronaphthalenes (1,2-DNO₂N; 1,8-DNO₂N) in nonpolar and polar solvents shows transient species with absorption maxima and lifetimes dependent on solvent polarity. In deaerated n-hexane the absorption maxima and lifetimes (1/K) are 490 nm and 1.0 μsec for 1,2-DNO₂N and 550 nm and 2.5 μsec for 1,8-DNO₂N. In deaerated ethanol the corresponding values are 550 nm and 4.3 μsec for 1,2-DNO₂N and 590 nm and 5.3 μsec for 1,8-DNO₂N. The transient absorptions are attributed to the lowest triplet excited states T₁ of the 1,2- and 1,8-DNO₂N. The observed red shifts in the absorption maxima of the T₁ states are indicative of the extent to which electronic charge is transferred intramolecularly during the T₁ → T_n transitions. Furthermore, the increased lifetime of the T₁ states with increasing solvent polarity indicates the intramolecular charge transfer character of the T₁ states. Changes of dipole moments accompanying the T₁ → T_n transitions as well as rate constants for electron or proton transfer and hydrogen abstraction reactions involving the T₁ states of 1,2- and 1,8-DNO₂N and tributyl tin hydride (Bu₃SnH) as the hydrogen donor were determined together with the activation energy of the hydrogen abstraction reaction for the case of 1,2-DNO₂N. The spectroscopic and kinetic data obtained in this work demonstrate that the triplet states of 1,2- and 1,8-DNO₂N behave like n → π* states in nonpolar media while in polar solvents the n → π* character of these states is reduced with a simultaneous increase in their intramolecular charge transfer character.     

One- and Two-Dimensional Torsion-Inversion Models for the Fluoral Molecule (CF3CHO) in Excited Electronic States

The structure of the conformationally nonrigid fluoral molecule (CF₃CHO) in the ground (S₀) and lowest excited triplet (T₁) and singlet (S₁) electronic states was studied by ab initio quantum-chemical methods. The equilibrium geometric parameters and harmonic vibrational frequencies of the molecule in these electronic states were determined. The calculations demonstrated that the electronic excitation causes substantial changes in the molecular structure involving the rotation of the CF₃ top and the deviation of the CCHO carbonyl fragment from planarity. The quantum-mechanical problems for large-amplitude vibrations, namely, for the torsional vibration in the S₀ state and the torsional and inversion vibrations (nonplanar carbonyl fragment) in the T₁ and S₁ states, were solved in the one- and two-dimensional approximations. A comparison of the results of calculations revealed the correlation between the torsional and inversion motions.     

Detection and characterization of recombinant DNA expressing <Emphasis Type="Italic">vip3A</Emphasis>-type insecticidal gene in GMOs—standard single,multiplex and construct-specific PCR assays

Vegetative insecticidal protein (Vip), a unique class of insecticidal protein, is now part of transgenic plants for conferring resistance against lepidopteron pests. In order to address the imminent regulatory need for detection and labeling of vip3A carrying genetically modified (GM) products, we have developed a standard single PCR and a multiplex PCR assay. As far as we are aware, this is the first report on PCR-based detection of a vip3A-type gene (vip-s) in transgenic cotton and tobacco. Our assay involves amplification of a 284-bp region of the vip-s gene. This assay can possibly detect as many as 20 natural wild-type isolates bearing a vip3A-like gene and two synthetic genes of vip3A in transgenic plants. The limit of detection as established by our assay for GM trait (vip-s) is 0.1%. Spiking with nontarget DNA originating from diverse plant sources had no inhibitory effect on vip-s detection. Since autoclaving of vip-s bearing GM leaf samples showed no deterioration/interference in detection efficacy, the assay seems to be suitable for processed food products as well. The vip-s amplicon identity was reconfirmed by restriction endonuclease assay. The primer set for vip-s was equally effective in a multiplex PCR assay format (duplex, triplex and quadruplex), used in conjunction with the primer sets for the npt-II selectable marker gene, Cauliflower mosaic virus 35S promoter and nopaline synthetase terminator, enabling concurrent detection of the transgene, regulatory sequences and marker gene. Further, the entire transgene construct was amplified using the forward primer of the promoter and the reverse primer of the terminator. The resultant amplicon served as a template for nested PCR to confirm the construct integrity. The method is suitable for screening any vip3A-carrying GM plant and food. The availability of a reliable PCR assay method prior to commercial release of vip3A-based transgenic crops and food would facilitate rapid and efficient regulatory compliance. Electronic supplementary material The online version of this article (doi:) contains supplementary material, which is available to authorized users. An application for an Indian patent (1891/DEL2006/17.08.07) comprising a substantive part of this study has been filed. ITRC communication no. 2516.     

Influence of containing moisture on hydrothermal stability of modified collagen thermal characteristics analysis by DSC

The thermal stability of sheepskin collagen cross-linked with chrome sulfate and mimosa (MI)–oxazolidine (OZ), respectively, had been researched in this experiment. All samples’ shrinkage temperatures (T _s) are determined by a special T _s-testing-apparatus and denaturation temperatures (T _d) are determined by the differential scanning calorimetry. The relations between the modified collagens containing moisture and their hydrothermal stability, T _s or T _d, were studied. The results show that the cross linking agents can enhance the thermal stability of modified collagen whose T _s are 109.8 and 110.6 °C for collagen treated with chrome and MI–OZ, respectively. When the samples contain 25–71.9% moisture for chrome leather and 20–71.1% for leather treated with MI–OZ, the hydrothermal stability will decrease with the increase of moisture. It was found that the difference between T _s and T _d of collagen modified by chrome is more obvious than that of collagen modified with MI–OZ. And when the moisture of chrome leather exceeds 55%, T _d cannot express thermal stability of modified collagen as a substitute for T _s, and the moisture is 40% for leather tanned with MI–OZ.     

A method for determining the mean translational energy of particles desorbed from solid surfaces

A method for determinig the mean molecular translational energy in gas flows of low intensity (10¹²–10¹⁴ molec. s^–1) has been proposed. The method was verified using various gases (H₂, N₂, O₂, and CO₂ flowing into a vacuum out of a heated capillary. The translational energies were determined for CO and N₂ molecules desorbing from the surface of polycrystalline Ir. The translational temperature (T _tr) measured for CO equals 650±90 K and almost coincides with the surface temperature (T _s = 600 K). In the case of nitrogen molecules,T _tr = 4600±500 K atT _s = 500 K. The method proposed is applicable to the determination of the spatial distribution of molecular beam particles.Translated fromIzvestiya Akademii Nauk. Seriya Khimicheskaya, No. 1, pp. 30–34, January, 1995.The authors express their gratitude to A. V. Sklyarov for fruitful discussions during the elaboration of the theoretical basis and technical realization of the method.The reseach was carried out with the partial financial support of the International Science Foundation (Grant MBN 000).