Cyclic nucleotide metabolism and reactive oxygen production by macrophages

The production of reactive oxygen species by elicited rat peritoneal macrophages was assessed by $\text{in vitro}$ measurement of chemiluminescence in the presence of luminol. The divalent ion ionophore A23187 stimulated the production of reactive oxygen species. This action was inhibited by monobutyryl and dibutyryl derivatives of cyclic AMP but was not affected by derivates of cyclic GMP. Cyclic AMP and cyclic GMP concentrations increased rapidly in macrophages exposed to A23187 or zymosan. Indomethacin (20 μmol/1) inhibited the increase in cyclic AMP concentration but not the increase in cyclic GMP concentration. Neither A23187 nor zymosan stimulated adenylate cyclase activity in broken cell preparations of macrophages. The observations are consistent with the hypothesis that PGE produced by macrophages after phagocytotic stimuli may inhibit certain macrophage functions and perform a regulatory role in these cells. This action of PGE may be mediated by cyclic AMP.     

A surprising new protein superfamily containing ovalbumin,antithrombin-III,and alpha1-proteinase inhibitor

A distant relationship between chicken ovalbumin and two human plasma protease inhibitors was revealed by computer analyses. We propose a new protein superfamily containing at least three families: ovalbumin (and probably gene X and gene Y proteins), antithrombin-III, and alpha₁-proteinase inhibitor. Although these families may have diverged from a common ancestor more than 500 million years ago, they may still share similarity in gene structure as well as in protein sequence.     

Control of pattern duplication in the retinotectal system of Xenopus. Suppression of duplication by eye-fragment interactions.

Recombining right nasal half-eyes with left temporal half-eyes at embryonic stage 32 in Xenopus produces a double or “twinned” pattern of functional connections between retina and midbrain optic tectum. The left temporal half-eye is reprogrammed such that it projects to the tectum as a mirror-image duplicate pattern of the nasal right half-eye; both half-eyes project across the entire tectum. However, recombining a right nasal half-eye (in situ) with a right dorsal half-eye (grafted into the temporal position; N_RD_R eye) produces a single normal retinotectal projection. Where interactions between N_R and T_L involve both axial reprogramming and duplication of N_R positional values in T_L, N_RD_R interactions involve axial reprogramming in D_R without duplication of N_R values. In a second approach to interactions which suppress pattern duplication, both nasal and temporal one-third-sized eye fragments form approximate “NN” or “TT” duplicate pattern maps, respectively, when either is allowed to round up and form a whole eye. Allowing nasal and temporal thirds to permanently fuse (after removal of a one-third-sized vertical center strip of retina at stage 32) produces a normal projection; allowing the nasal and temporal thirds to interact (fuse) for 35–40 hr, followed by removal of one or the other third, suppresses pattern duplication (produces normal maps) in the remaining third in a majority of cases. Allowing the thirds to interact for 18–30 hr before removal of the temporal third produces a majority result of partial duplication in the remaining nasal third. Partial duplicates are apparent spatial intermediates with regard to interactions which suppress duplication in either fragment type.     

Release of gastrin by vagal stimulation in the acid secretory response to food.

Gastric pouches were constructed in 8 dogs; in 4 they were of denervated type and in 4 the innervation was intact. An oesophageal fistula was then prepared in each dog. The acid secretory response to oral, tube and sham feeding was determined before and after denervation of the pyloric antrum. The results support the view that vagal release of gastrin makes a relatively small contribution to the total acid secretory response to food.     

Cryopreservation of human granulocytes.

Granulocyte preservation was undertaken using hydroxyethylstarch for both sedimentation of red cells and cryopreservation of buffy coat white cells from CPD whole blood. Buffy coats were mixed with HES to a final concentration of 4% (w/v) and hematocrit of 30%, and sedimented in inverted plastic syringes. The leukocyte enriched (100–500×) supernatant was frozen at 2.0 °C/min to ?80 °C (and stored frozen up to 3 months). Alternatively, sedimented leukocytes were frozen after a slow addition of 10% DMSO to 5%. Tubes were thawed at 37 °C, and DMSO was removed by dilution with Hank's solution containing CPD and centrifugation. The pellets of granulocytes were resuspended in Normosol.Buffy coat from 10 units yielded 60 ± 9.7% of the available whole blood leukocytes, of which 43 ± 14% were recovered after sedimentation in HES. Freezing in DMSO yielded all, 101% of the prefrozen leukocytes. Postthawed viability of granulocytes was estimated morphologically and by their ability to inhibit the rate of growth of E. coli. Complete inhibition was observed at a ratio of one E. coli to one granulocyte. Postthawed granulocytes were characterized by high myeloperoxidase activity and exclusion of trypan blue. Approximately 25% of the total available granulocytes in CPD whole blood were recovered.     

Organismal differences in post-translational modifications in histones H3 and H4

Post-translational modifications (PTMs) of histones play an important role in many cellular processes, notably gene regulation. Using a combination of mass spectrometric and immunobiochemical approaches, we show that the PTM profile of histone H3 differs significantly among the various model organisms examined. Unicellular eukaryotes, such as Saccharomyces cerevisiae (yeast) and Tetrahymena thermophila (Tet), for example, contain more activation than silencing marks as compared with mammalian cells (mouse and human), which are generally enriched in PTMs more often associated with gene silencing. Close examination reveals that many of the better-known modified lysines (Lys) can be either methylated or acetylated and that the overall modification patterns become more complex from unicellular eukaryotes to mammals. Additionally, novel species-specific H3 PTMs from wild-type asynchronously grown cells are also detected by mass spectrometry. Our results suggest that some PTMs are more conserved than previously thought, including H3K9me1 and H4K20me2 in yeast and H3K27me1, -me2, and -me3 in Tet. On histone H4, methylation at Lys-20 showed a similar pattern as H3 methylation at Lys-9, with mammals containing more methylation than the unicellular organisms. Additionally, modification profiles of H4 acetylation were very similar among the organisms examined.     

Low seed availability may limit recruitment in grazed Atriplex vesicaria and contribute to its local extinction

Poor recruitment in Atriplex vesicaria Hewd exBenth (bladder saltbush) under sheep grazing in the chenopodshrublands of southern Australia contributes to a decline in the shrub'spopulation growth rate. This may lead to local extinction of the species overlarge areas around watering points. This study investigated whether low seedavailability may contribute to poor recruitment. It examined the incidence offlowering and seed bank size at sites distributed across a large grazedpaddock,and examined the longevity of seed in the soil. Grazing by sheep reduced theincidence of flowering and input to the seed bank. The proportion of shrubswithflowers increased with distance from water, showing the characteristicpiosphereresponse. Shrubs on grazed sites closer to water experienced extended periodswhen they failed to flower or flowered poorly. The seed bank was negligible atthree of the sites within 1650 m of water for all three years ofsampling. In contrast, the seed bank at the most distant site sampled (2800m from water) was small in 1990 (37 ± 5.1seeds/m²) but in 1991 and 1992 seed numberswere substantial (626 ± 315.2 seeds/m²and 318 ± 169.0, respectively). Soil seed was short-lived inthis study, with only 34% and 17% of the original seed remainingas viable ungerminated seed after 12 months for the under-canopy andexposed treatments respectively. Whilst recruitment may also be limited byaltered soil conditions due to grazing and trampling and the availability ofsafe sites, the results of this study suggest that low seed availability may bean important factor contributing to poor recruitment and may limit the abilityof the population to recover from the loss of established plants. Management ofgrazing must take into account the need for A. vesicariapopulations to flower and set seed on a regular basis.