Distribution of sarcoplasmic reticulum Ca-ATPase and of calsequestrin in rabbit and rat skeletal muscle fibers

Summary Muscle fibers in rabbit extensor digitorum longus (EDL), tibialis anterior (TA) and soleus, and rat soleus, were examined immunohistochemically for two proteins of the sarcoplasmic reticulum, Ca-ATPase and calsequestrin (CaS). Fibers were typed with the histochemical reaction for actomyosin ATPase. In the rabbit EDL and TA, type I fibers clearly reacted less for Ca-ATPase and CaS than type II fibers, but the difference was less with CaS than with Ca-ATPase. Although the differences were relatively small, HB fibers consistently presented greater amounts of Ca-ATPase than IIA fibers. No types II subgroups could be recognized after incubation with anti-CaS. These findings confirm results from previous immunochemical measurements on whole muscles containing different proportions of IIA and IIB fibers (Leberer and Pette 1986). Type IIA and IIC in the rabbit and rat soleus reacted stronger for Ca-ATPase and for CaS than type I fibers. Small differences in Ca-ATPase, but not in CaS, were recognized within the type I fiber population. Therefore, type I fibers in the rabbit and rat soleus are not a homogeneous population.     

Nif- Hup- mutants of Rhizobium japonicum.

Two H2 uptake-negative (Hup-) Rhizobium japonicum mutants were obtained that also lacked symbiotic N2 fixation (acetylene reduction) activity. One of the mutants formed green nodules and was deficient in heme. Hydrogen oxidation activity in this mutant could be restored by the addition of heme plus ATP to crude extracts. Bacteroid extracts from the other mutant strain lacked hydrogenase activity and activity for both of the nitrogenase component proteins. Hup+ revertants of the mutant strains regained both H2 uptake ability and nitrogenase activity.     

The effect of calmodulin and far-red light on the kinetic properties of the mitochondrial and microsomal calcium-ion transport system from corn

The kinetic properties of active Ca²⁺ transport into mitochondria and microsomal membrane vesicles prepared from coleoptiles of dark-and light-grown corn seedlings have been studied. The apparent values for K _m and V _max for Ca²⁺ of the mitochondrial transport system from dark-grown plants are about one order of magnitude higher than those from the microsomal transport system. Calmodulin has no effect on the Ca²⁺ accumulation into mitochondria whereas the apparent maximum transport velocity and affinity for Ca²⁺ of the microsomal Ca²⁺-transport system are both increased by calmodulin. When intact corn seedlings are irradiated with far-red light, the calmodulin-induced increase of the apparent maximum transport velocity and affinity for Ca²⁺ can no longer be observed. From these data it can be concluded that the low cytoplasmic Ca²⁺ concentration in the cytoplasm of coleoptile cells from dark-grown corn is maintained by a calmodulin-regulated Ca²⁺ pump. Irradiation with photomorphogenically active far-red light lowers the Ca²⁺-transport activity and thus causes an increase of the cytoplasmic, free-Ca²⁺ concentration. The physiological implications will be discussed.     

Effect of ethylenediamine di (o-hydroxyphenylacetic acid) application to soil columns on the distribution of certain nutrient elements in the water-soluble,acid-soluble and exchangeable forms

Summary The chemical behaviour of the sodium form of ethylenediamine di(o-hydroxyphenylacetic acid), Na₂EDDHA, in a calcareous soil column was studied. The results show loss about 2/3 of the synthetic chelate in the soil, possibly due to microbial decomposition and/or fixation of EDDHA. The application of Na₂EDDHA caused an increase in the amount of water-soluble forms of certain elements in the following decreasing order: Fe, Cu, Mn, Ni, Zn and Ca. The increase in the water-soluble forms of such elements is due possibly to the chelation of their insoluble compounds in the soil. The solubilization effect of Na₂EDDHA and the subsequent movement of the elements in the soil solution resulted in a significant decrease in their amounts in the exchangeable and acid-soluble forms in the soil. In conclusion, the synthetic chelate of EDDHA underwent chemical reactions in the soil and caused changes in the ratio of certain elements in the various chemical forms. Sen. author, formerly graduate student at the University of Arizona, now Assistant Professor, University of Ain-Shams, Cairo, Egypt. Jr. author, Vice Chancellor, University of Wisc.-Green Bay.     

Immune response genes in inbred rats. II. Segregation studies of the GT and GA genes and their linkage to the major histocompatibility locus

Genetic analysis of the high responder-non-(or low) responder differences between WF and ACI rats to the synthetic copolymers GT and GA established singleIr-genes for both antigens and dominance for high responder status.Ir-GT andIr-GA are linked to the major histocompatibility locus. It could be demonstrated that only T cells carrying the high responderIr-GT gene undergo in vitro blast transformation to GT. The advantages of the rat systems for further studies of the regulatory role ofIr-genes on the cellular level are discussed.Abbreviations cpm counts per minute - DHR delayed hypersensitivity reaction - GA random synthetic copolymer of L-glutamic acid⁵⁰, L-alanine⁵⁰, M.W. 45,000 - GT random synthetic copolymer of L-glutamic acid⁵⁰, L-tyrosine⁵⁰, M.W. 22,000 - Ir gene immune response gene - MLC mixed lymphocyte cultures - LDH lactic dehydrogenase - (T,G)-A-L branched chain synthetic polymer of poly-L (tyrosine, glutamic acid)-poly-D, L-alanine-poly-L-lysine Rat Strains ACI ACI/MaI - WF Wistar Furth - AUG August 28807/Cr     

Enzymatic methylations: III. Cadaverine-induced conformational changes of E.coli tRNAfMet as evidenced by the availability of a specific adenosine and a specific cytidine residue for methylation+

A partially purified tRNA methylase fraction from rat liver, containing m(2)G- m(1)A- and m(5)C-methylase, was used to study the influence of Mg(++) and of the biogenic polyamine cadaverine on the enzymatic methylation of E.coli tRNA(fMet)in vitro. In presence of 1 or 10 mM Mg(++), guanosine no. 27 was methylated to m(2)G. In 1 mM Mg(++) plus 30 mM cadaverine, guanosine in position 27 and adenosine in position 59 were methylated. In presence of 30 mM cadaverine alone tRNA(fMet) accepted three methyl groups: in addition to guanosine no. 27 and adenosine no. 59 cytidine no. 49 was methylated. In order to correlate tRNA(fMet) tertiary structure changes with the methylation patterns, differentiated melting curves of tRNA(fMet) were measured under the methylation conditions. It was shown that the thermodynamic stability of tRNA(fMet) tertiary structure is different in presence of Mg(++), or Mg(++) plus cadaverine, or cadaverine alone. From the differentiated melting curves and from the methylation experiments one can conclude that at 37 degrees in the presence of Mg(++) tRNA(fMet) has a compact structure with the extra loop and the TpsiC-loop protected by tertiary structure interactions. In Mg(++) plus cadaverine, the TpsiC-loop is available, while the extra loop is yet engaged in teritary structure (G-15: C-49) interactions. In cadaverine alone, the TpsiC-loop and the extra loop are free; hence under these conditions the open tRNA(fMet) clover leaf may be the substrate for methylation. In general, cadaverine destabilizes tRNA tertiary structure in the presence of Mg(++), and stabilizes tRNA(fMet) tertiary structure in the absence of Mg(++). This may be explained by a competition of cadaverine with Mg(++) for specific binding sites on the tRNA. On the basis of these experiments a possible role of biogenic polyamines in vivo may be discussed: as essential components of procaryotic and eucaryotic ribosomes they may together with ribosomal factors facilitate tRNA-ribosome binding during protein biosynthesis by opening the tRNA tertiary structure, thus making the tRNA's TpsiC-loop available for interaction with the complementary sequence of the ribosomal 5S RNA.     

Differential staining of plant chromosomes with Giemsa

Simple Giemsa staining techniques for revealing banding patterns in somatic chromosomes of plants are described. The value of the methods in the recognition of heterochromatin was demonstrated using five monocotyledonous and two dicotyledonous species. In Trillium grandiflorum the stronger Giemsa stained chromosome segments were shown to be identical with the heterochromatic regions (H-segments) revealed by cold treatment. Preferential staining of H-segments was also observed in chromosomes from three species of Fritillaria and in Scilla sibirica. Under suitable conditions the chromosomes of Vicia faba displayed a characteristic banding pattern and the bands were identified as heterochromatin. The Giemsa techniques proved to be more sensitive than Quinacrine fluorescence in revealing a longitudinal differentiation of the chromosomes of Crepis capillaris, where plants with and without B-chromosomes were examined. Again all chromosome types had their characteristic bands but there was no difference in Giemsa staining properties between the B-chromosomes and those of the standard complement.