Expression of antisense nodulin-35 RNA in Vigna aconitifolia transgenic root nodules retards peroxisome development and affects nitrogen availability to the plant

A nodulin-35 (N-35) cDNA encoding nodule-specific uricase (EC 1.7.3.3.) was isolated from a Vigna aconitifolia (mothbean) root nodule cDNA library. Sequence analysis of Vigna uricase (VN-35) cDNA revealed 90% homology to that of soybean. The VN-35 cDNA was inserted in the antisense orientation downstream of the CaMV—35S promoter, and transgenic hairy roots were formed on Vigna plants using Agrobacterium rhizogenes . Infection with Bradyrhizobium (cowpea) gave rise to root nodules on transgenic hairy roots supported by the wild-type shoot. Expression of antisense VN-35 RNA was detected in transgenic nodules on individual roots using polymerase chain reaction (PCR). The nodules expressing antisense VN-35 RNA were smaller in size and showed lower uricase activity than nodules formed on the hairy roots transformed with a binary vector containing β-glucuronidase (GUS) gene (used as control), and the plants exhibited nitrogen deficiency symptoms. Ultrastructural analysis and immunogold labeling with antibody against soybean N-35 revealed that the growth of peroxisomes was retarded in transgenic nodules expressing antisense VN-35 RNA. These data suggest that a reduction in ureide biosynthesis limits the availability of symbiotically reduced nitrogen to the plant. The nodules of tropical legumes appear to be specialized in nitrogen assimilation and are developmentally controlled to produce and transport ureides.     

A tumor cell line producing granulocyte colony-stimulating factor and an immune suppressive factor

From a patient, both a cell line incapable of secreting granulocyte colony-stimulating factor (G-CSF) (TC873) and a cell line capable of secreting G-CSF (TCM902) were established. The effector cells induced, with TC873 cells showed a high lytic capacity against two types of tumor cells. The effector cells induced by TCM902 cells did not show such capacity. Furthermore, the TCM902 cells excreted a factor suppressing the proliferation of lymphokine activated killer (LAK) cells and the autologous tumor cell lysis of tumor associated lymphocytes. This factor probably is TFG- ₁.Abbreviations CSF colony stimulating factor - ELISA enzyme-linked immunosorbent assay - G granulocyte - GM granulocyte-monocyte - IFN interferon - IL interleukin - LAK lymphokine activated killer - M monocyte - MLTC mixed lymphocyte tumor cell culture - TGF transforming growth factor - TILs tumor infiltrating lymphocytes - TNF tumor necrosis factor     

Picosecond Raman spectroscopy of the B830 LH2 complex ofChromatium purpuratum BN 5500

A setup for generating the Stokes Raman lines of benzene (556, 588 and 624 nm, 50 ps) by the use of the second harmonic of a Nd: YLF regenerative amplifier system (527 nm, 70 ps, 1 kHz) has been built. This was then used to detect, for the first time, the picosecond Raman spectrum of a carotenoid bound to an isolated light-harvesting complex of a photosynthetic bacterium. The 527 and 588 nm pulses have been used, respectively, for pumping and probing (delay 0 ps) the S₁ and T₁ states of okenone which is bound to both the isolated B830 LH2 complex and the chromatophores fromChromatium purpuratum BN 5500. Comparison of the above spectra with the S₁ and T₁ Raman spectra of all-trans-okenone, free inn-hexane solution, shows that only the T₁ state is detected with the LH2 complex, and that both the S₁ and T₁ states are detected with the chromatophores. The results indicate that in the chromatophores there are at least two types of S₁ carotenoids with different lifetimes, i.e., one in the LH2 complex which is too short-lived to be detected, most probably due to efficient energy transfer to bacteriochlorophyll, and the other in either the reaction center or the LH1 complex which is long-lived enough to be pumped and probed by 50 70 ps pulses. The results also indicate that at least two of the actively light-harvesting carotenoid molecules are in close connection in the isolated LH2 complex since the T₁ state is generated through singlet homofission within the short S₁ lifetime.     

Effects of acidic pH on the formation of vinblastine-induced paracrystals in Chinese hamster ovary cells

Summary— The pH-related change in morphology of vinblastine (VLB)-induced paracrystals formed in Chinese hamster ovary (CHO) cells was examined immunohistochemically in order to determine both the mechanism of tubulin crystallization and the influence of acidic pHs on cytoskeletal microtubules. Lowering the extracellular pH (pHe) rapidly reduced the intracellular pH (pHi) in CHO cells. Lowering the pHi to near the neutral range significantly accelerated the growth of VLB-induced paracrystals, compared to that of paracrystals formed at a physiological pHe. However, further cytoplasmic acidification caused by the addition of sodium azide into the culture medium induced the disappearance of typical paracrystals and the appearance of a highly organized meshwork of tubulin appearing as short, thick filaments at the light microscopic level. Treatments using different concentrations of VLB at different pHe's showed that low pHi's (6.7 and 6.3) suppressed paracrystal-formation at lower concentrations of VLB (5×10^?6 M and 10^?5 M). At higher concentrations of VLB (5×10^?5 M and 10^?4 M), only short filaments were formed at pHi 6. 3. Electron microscopy revealed that the filaments had a ladder-like structure probably consisting of a stacked series of fused rings. This indicates that paracrystals may be modified by extremely low pH. These results show that paracrystals are unstable in living cells and that their formation is regulated by environmental pH.     

Oxidative Bioconversion of Cholesterol by Pseudomonas sp. Strain ST-200 in a Water-Organic Solvent Two-Phase System

Pseudomonas sp. strain ST-200, which is capable of conversion of cholesterol, was isolated from humus soil. This organism effectively modified cholesterol dissolved in an organic solvent by dehydrogenation and oxygenation. When the organism was grown in a medium overlaid with a 10% volume of a mixed organic solvent (p-xylene and diphenylmethane; 3:7, vol/vol) containing cholesterol (20 mg/ml), the cholesterol concentration in the organic solvent was reduced to only 0.4 mg/ml after 8 days. Although the organism did not assimilate cholesterol, 98% of the cholesterol initially present disappeared. The organic solvent layer contained two major and three minor compounds converted from cholesterol. The major compounds were 6β-hydroxycholest-4-en-3-one (8.9 mg/ml) and cholest-4-ene-3,6-dione (7.6 mg/ml). The concentrations of these compounds were equivalent to 43 and 37% of the cholesterol initially present. This organism would provide an effective and convenient system to oxidize the C-3 and -6 positions of cholesterol by introduction of a hydroxyl or ketone group.     

Spectral sensitivities of jumping spider eyes

Summary Spectral sensitivities of the anterior lateral, posterior lateral and anterior median eyes of the jumping spider,Menemerus confusus Boes. et Str. have been studied by recording electroretinograms (ERGs) and receptor potentials. The anterior and posterior lateral eyes have a single type of visual cell with a maximum spectral sensitivity at about 535–540 nm. The anterior median eye has four types of visual cells with maximum sensitivities at about 360, 480–500, 520–540 and 580 nm, respectively. The ERGs recorded from the optic nerve side (posterior part of the retina) were affected greatly by long wave chromatic light and those on the corneal side (anterior part of the retina) by short wave chromatic light, suggesting that each receptor layer contains a different photopigment.     

The enhanced production of hyaluronic acid by cultured rat fibroblast cells treated with cyclic AMP and its dibutyryl derivative

Cells of a newly established rat fibroblast line (SEN) in culture synthesize mucopolysaccharides, which have been identified as hyaluronic acid, chondroitin-4-sulfate and heparan sulfate. Treatment of the cells with adenosine 3′:5′-cyclic monophosphate resulted in a marked stimulation of production of hyaluronic acid, but not of the other mucopolysaccharides. Treated cells also showed increased activity of hyaluronic acid synthetase, a reduction in growth rate, and morphological alteration. In addition, 5-bromodeoxyuridine was found to counteract greatly the cyclic AMP effect.     

Salinity tolerance and structure of external and internal gills in tadpoles of the crab-eating frog,Rana cancrivora

Summary Salinity tolerance and histology of gills were studied in Rana cancrivora larvae. The tadpoles at the external gill stages (W stages 21–22) were able to survive in media containing up to 40% seawater, but died in water of higher salinity. Their external gills appear to have no critical role in adaptation to seawater. However, advanced tadpoles with internal gills (T-K stages I–XVIII) were able to tolerate 50% or higher seawater. In the internal gills, there are numerous mitochondriarich cells (MR cells) scattered on the ventral and lateral epithelia of the gill arches and the gill tufts in both freshwater-and seawater-acclimated tadpoles. In freshwater-acclimated tadpoles there are three types of MR cell: (1) microplicated, (2) microvillous, and (3) apically vacuolated. In tadpoles acclimated to dilute seawater, the ratio of type-1 to type-2 cells is lower, although all three types of MR cell are present. In 60%-seawater-acclimated tadpoles, a few MR cells with a lumen and concave cytoplasm at the apical membrane (type 4) are present. The changes in MR cell morphology under ambient conditions of low or high salinity may reflect alterations in the physiological roles of the gills with regard to transport of ions.     

Equilibrium swelling of pigment gallstones: Evidence for network polymer structure

A major component of pigment gallstones (PS) is a black, insoluble substance. It has been suggested that this pigment material might be a highly crosslinked polymer, and if such were the case, it should imbibe solvent (swell) to the maximum permitted by the crosslinks of its macromolecular network. We measured the equilibrium amount, q_eq, by which pulverized, desiccated PS swells in different liquids, including isotonic aqueous buffers at pH values from 1.5–11.5. For ionic strengths ≥ 0.15, the dependence of q_eq on pH exhibits a broad titration curve with a midpoint near pH 7. q_eq was < 1.2 in methanol, dimethylformamide, dimethylsulfoxide, and chloroform. The ir absorbance from vinyl groups in the black pigment was only one-eighth that of unconjugated bilirubin, the primary chemical building block of PS; this implicates vinyl groups in the formation of a polymer network. The rise in q_eq with increasing pH suggests that the carboxyl groups are free to ionize and are therefore not involved in the covalent bonds that make the crosslinked polymer. A network polymer structure would account for the inability to dissolve PS in those solvents in which unconjugated bilirubin is soluble.