Correlative Inhibition of Lateral Bud Growth in Pisum sativum L. and Phaseolus vulgaris L.: Studies of the Role of Abscisic Acid

The possibility has been investigated that abscisic acid (ABA)might act as a correlative inhibitor of lateral bud growth inPisum sativum and Phaseolus vulgaris. Application of ABA insmall quantities (2µg) to axillary buds on decapitatedplants of P. sativum caused appreciable inhibition of theirgrowth, and induced a compensatory growth of the bud on an adjacentnode. Application of this same quantity of ABA to axillary budson decapitated plants of Phaseolus vulgaris was without effect,but a high concentration in lanolin (1 mg g^–1) did substantiallyreduce bud outgrowth. Endogenous ABA-like substances in Phaseolusvulgaris, detected by bioassay and electron capture g.l.c.,were present in similar concentrations in shoot tips, lateralbuds on intact plants and lateral buds on plants decapitated24 h earlier. The effects of applied ABA suggested that it might be involvedin the mechanism of correlative inhibition in Pisum sativum,but it was not possible to test this hypothesis by determiningendogenous ABA levels in axillary buds because of their smallsize. The evidence presented here suggests that ABA is not acorrelative inhibitor in Phaseolus vulgaris even though at highconcentration it can inhibit the growth of axillary buds.     

橙花瑞香的繁殖特性研究

瑞香属植物具有重要的药用和观赏价值,在中国资源丰富,但自然条件下低坐果率限制了该属植物的进一步开发和利用。该研究以橙花瑞香为对象,通过对其有性繁殖及传粉特性的研究,探索其自然坐果率低的原因,内容包括花部特征的测量分析,MTT染色法测定花粉活性,联苯胺-过氧化氢法测定柱头可授性,扫描电镜观察柱头、花粉的形态,传粉者观察,通过花粉胚珠比(P/O)和人工授粉实验推测橙花瑞香的繁育系统类型。结果表明:橙花瑞香的花部结构特殊,管状小花,花药两轮,雌雄蕊分离。花开后的花粉具有活性,柱头具有可授性,扫描电镜下,柱头和花粉的结构没有发育异常,且柱头上有花粉落置。橙花瑞香的传粉者主要是夜间访花的蛾类,访花频率低。P/O及人工授粉实验表明橙花瑞香的繁育系统为专性异交。橙花瑞香的坐果率非常低,自然坐果率为1.4%,人工异花授粉为23.3%,低坐果率可能是受其开花量大、异花花粉限制、资源限制以及花部结构等因素的影响。     

The enigmatic truffle Fevansia aurantiaca is an ectomycorrhizal member of the Albatrellus lineage

Fevansia aurantiaca is an orange-colored truffle that has been collected infrequently in the Pacific Northwest of the USA. This sequestrate, hypogeous fungus was originally thought to be related to the genera Rhizopogon or Alpova in the Boletales, but the large, inflated cells in the trama and the very pale spore mass easily segregated it from these genera. To date, no molecular phylogenetic studies have determined its closest relatives. F. aurantiaca was originally discovered in leaf litter beneath Pinaceae, leading Trappe and Castellano (Mycotaxon 75:153–179, 2000) to suggest that it is an ectomycorrhizal symbiont of various members of the Pinaceae. However, without direct ecological or phylogenetic data, it is impossible to confirm the trophic mode of this truffle species. In this study, we combined phylogenetic analysis of the ITS and 28S ribosomal DNA with data on microscopic morphology to determine that F. aurantiaca is a member of the Albatrellus ectomycorrhizal lineage (Albatrellaceae, Russulales).     

Boron Mobility in Two Coniferous Species

In contrast to earlier beliefs, it is now known that boron (B)can be retranslocated complexed with sugar alcohols in someplant species. Conifers had been thought not to translocatesugar alcohols in the phloem. However, 1 d after applying¹⁰Benriched boric acid to shoots of Scots pine and Norway spruceseedlings, we found increases in both the amount and proportionof¹⁰B in the root systems in both species. We conclude thatB is translocated in the phloem from shoots to roots in spruceand pine, and therefore it is possible that these species retranslocateB. Copyright 2000 Annals of Botany Company Scots pine, Pinus sylvestris, Norway spruce, Picea abies, conifers, boron retranslocation, roots, stable isotopes, sugar alcohols, boron complexes, mineral nutrition, forest trees     

Respiration and Mitochondrial Activity in Zea mays Roots As Affected by Osmotic Stress

Studies were made of metabolism in highly vacuolated and slightlyvacuolated Zea mays root tissue both during and after plasmolysis. Plasmolysis resulted in decreased respiration and carbon dioxideevolution from glucose and an increased sucrose synthesis. Inhibitionof respiration during plasmolysis in both the highly vacuolatedand slightly vacuolated tissue was not relieved by supply ofglucose, organic acids, or uncouplers of oxidative phosphorylation.Mitochondria isolated from plasmolysed tissue were tightly coupled,but activity in vitro was inhibited by exposure to a high negativeosmotic potential. It is suggested that low TCA cycle activityin vivo must be due either to inhibition of mitochondrial activityor to reduced flow of carbon through the glycolytic pathway. A low potential for TCA cycle activity after deplasmolysis issuggested, as addition of pyruvate stimulated carbon dioxideevolution but not oxygen uptake, which was severely decreased.This was presumably due to severe mitochondrial damage as shownby their activity in vitro. However, it is not clear whetherrespiration in vivo is rate limited by rapid leakage of metabolicintermediate (reported earlier) or by lysis of mitochondria. Deplasmolysis did not damage mitochondria from slightly vacuolatedtissue, a result which was consistent with respiratory measurementsmade in vivo. The data show that mitochondria in vacuolated tissue are damagedduring and after deplasmolysis and not before. It is suggestedthat lysis of mitochondria occurs in vivo as a result of a sharpincrease in the osmotic potential of the cell fluids.     

Mitogenomics of Vetigastropoda: insights into the evolution of pallial symmetry

The nucleotide sequences of the complete or nearly complete mitochondrial (mt) genomes of seven vetigastropods were determined: Angaria neglecta (Angarioidea), Phasianella solida (Phasianelloidea), Granata lyrata (Seguenzioidea), Tegula lividomaculata and Bolma rugosa (Trochoidea), Diodora graeca (Fissurelloidea) and Lepetodrilus schrolli (Lepetodriloidea). While the mt genomes of the superfamilies Angarioidea, Phasianelloidea, Seguenzioidea and Trochoidea conform generally to the ancestral gene order of Vetigastropoda and Gastropoda, those of the superfamilies Fissurelloidea and Lepetodriloidea have suffered important rearrangements. The gene order of the mtDNA of Chrysomallon squamiferum, a representative of Neomphalina, was also analysed since it has been proposed to be closely related to Vetigastropoda, and showed a distinct arrangement. The reconstructed phylogenies recovered Neomphalina as a distinct gastropod lineage that is the sister group (only with moderate bootstrap support) of a clade including Vetigastropoda and Neritimorpha + Caeno‐gastropoda while the relative position of Heterobranchia and Patellogastropoda in the gastropod tree could not be determined definitively due to their long branches. Within the monophyletic Vetigastropoda, the superfamily Fissurelloidea was recovered as the sister group of two lineages, one including Lepetodriloidea as the sister group of Seguenzioidea + Halitoidea, the other including Phasianelloidea, Angarioidea and Trochoidea without resolved relationships. The long branches of Fissurelloidea were found to introduce significant tree instability in phylogenetic reconstruction. The new phylogeny supports that the loss of the right pallial gill occurred multiple times in vetigastropod evolution as previously suggested and that Phasianelloidea, Angarioidea and Trochoidea radiated from a common asymmetric (single‐gilled) ancestor that lived in the middle Palaeozoic.     

Atebbania Bernasconii, a New Genus and Species from Subterranean Waters of the Tiznit Plain, Southern Morocco (Gastropoda: Hydrobiidae)

The new genus Atebbania is described for a new hydrobiid species,A. bernasconii, which lives in groundwaters of southern Morocco.Of the Hydrobiidae genera with known shell and anatomy Moitessieriais the closest to Atebbania. The two share the following characters:shell elongate; teleoconch surface with evident microsculpture;seminal receptacle absent. Atebbania is distinguished from Moitessieriaby: shell ovate; penis with a) apical stylet, b) one lobe bentdownward on left (inner) side and c) penial duct running nearthe right (outer) side; posterior end of foot indented. Atebbaniabernasconii n. sp., lives in a limited area, the Tiznit plainin southern Morocco. Other stygobiont hydrobiids from otherareas of Morocco are currently being studied. None of them appearsto be closely related to A. bernasconii or to the species ofMoitessieria (Received 10 February 1998; accepted 30 April 1998)     

Polyamines in plants infected by citrus exocortis viroid or treated with silver ions and ethephon

The levels of polyamines in leaves of Gynura aurantiaca DC and tomato, Lycopersicon esculentum Mill. cv Rutgers, infected with citrus exocortis viroid (CEVd) or treated with silver nitrate or ethephon (2-chloroethylphosphonic acid) were measured by HPLC in relation to development of symptoms. Previously it had been demonstrated that treatment of G. aurantiaca plants with silver nitrate or ethephon closely mimicked the effects of viroid infection in the plants. In the studies reported here, a marked decrease in putrescine level was observed in plants infected by CEVd or treated with silver ions or ethephon. There was no significant change in either spermidine or spermine levels. Treatment of G. aurantiaca plants with specific inhibitors of ethylene biosynthesis (aminoethoxyvinylglycine, Co²⁺) or ethylene action (norbornadiene) prevented the decrease of putrescine associated with silver nitrate treatment and had no effect on spermidine or spermine levels. The development of viroid-like symptoms, the production of associated pathogenesis-related proteins, and the rise in protease activity induced by silver nitrate, were all suppressed by exogenous application of putrescine. The decreased level of putrescine as an ethylene-mediated step in the transduction of the viroid and silver or ethephon signaling is discussed.     

Musa aurantiaca (Musaceae) and its intraspecific taxa in India

Musa aurantiaca Baker (Musaceae) is distributed from northeast India, Tibet to northern Myanmar. In the present study its intraspecific taxa are thoroughly investigated. Two new varieties are described and illustrated based on live plants in the field: M. aurantiaca Baker var. homenborgohainiana Gogoi and M. aurantiaca Baker var. jengingensis Gogoi. A key to the varieties of Musa aurantiaca Baker and closely related taxa is also provided.     

Cross-linking Phytochrome to its Receptor in situ using Imidoesters

Phytochrome can be cross-linked to a particulate fraction usingimidoesters, namely dimethy adipimidate (DMA) and dimethyl suberimidate(DMS). DMS was more effective than DMA. Cross-linking of phytochrometo its in situ receptor effected by DMS occurred in red light-irradiatedcoleoptiles. If DMS cross-linking was carried out prior to redlight irradiation there was very little formation of particulatephytochrome. Phytochrome in the particulate fraction obtainedby in situ DMS cross-linking was totally resistant to the solubilizingeffect of washing with solutions of high salt concentrationand high pH and was indistinguishable spectro-scopically fromthe phytochrome in untreated coleoptiles. DMS cross-linkingof phytochrome to its assumed receptor in situ preferentiallyprotected it from destruction following red light irradiationand also prevented it from dissociating from its receptor followingR/FR¹ irradiation when incubated subsequently in the dark. Thesecharacteristics of phytochrome in DMS-treated coleoptiles matchedthose observed using glutaraldehyde as the cross-linking reagent.It is therefore concluded that earlier results obtained usingglutaraldehyde are not peculiar to that reagent and can be duplicatedreadily using more defined bifunctional cross-linkers.     

Cytosolic pH regulates GCl through control of phosphorylation states of CFTR

Our objective inthis study was to determine the effect of changes in luminal andcytoplasmic pH on cystic fibrosis transmembrane regulator (CFTR)Cl conductance(G_Cl). Wemonitored CFTRG_Cl in the apicalmembranes of sweat ducts as reflected byCl diffusion potentials(V_Cl) andtransepithelial conductance(G_Cl). We foundthat luminal pH (5.0-8.5) had little effect on thecAMP/ATP-activated CFTRG_Cl, showing thatCFTR G_Cl ismaintained over a broad range of extracellular pH in which it functionsphysiologically. However, we found that phosphorylation activation ofCFTR G_Cl issensitive to intracellular pH. That is, in the presence of cAMP and ATP [adenosine5'-O-(3-thiotriphosphate)],CFTR could be phosphorylated at physiological pH (6.8) but not at lowpH (~5.5). On the other hand, basic pH prevented endogenousphosphatase(s) from dephosphorylating CFTR.After phosphorylationof CFTR with cAMP and ATP, CFTRG_Cl is normallydeactivated within 1 min after cAMP is removed, even in the presence of5 mM ATP. This deactivation was due to an increase in endogenousphosphatase activity relative to kinase activity, since it was reversedby the reapplication of ATP and cAMP. However, increasing cytoplasmicpH significantly delayed the deactivation of CFTRG_Cl in adose-dependent manner, indicating inhibition of dephosphorylation. Weconclude that CFTRG_Cl may beregulated via shifts in cytoplasmic pH that mediate reciprocal controlof endogenous kinase and phosphatase activities. Luminal pH probably has little direct effect on these mechanisms. This regulation of CFTRmay be important in shifting electrolyte transport in the duct fromconductive to nonconductive modes.

     

Functional upregulation of H+-ATPase by lethal acid stress in cultured inner medullary collecting duct cells

The response ofH⁺-ATPase to lethal acid stress isunknown. A mutant strain (called NHE2d) was derived from cultured inner medullary collecting duct cells (mIMCD-3 cells) following three cyclesof lethal acid stress. Cells were grown to confluence on coverslips,loaded with2',7'-bis(carboxyethyl)-5(6)-carboxyfluorescein, andmonitored for intracellular pH(pH_i) recovery from an acid load. The rate of Na⁺-independentpH_i recovery from an acid load inmutant cells was approximately fourfold higher than in parent cells(P < 0.001). TheNa⁺-independentH⁺ extrusion was ATP dependent and K⁺ independent and wascompletely inhibited in the presence of diethylstilbestrol, N, N'-dicyclohexylcarbodiimide,or N-ethylmaleimide. Theseresults indicate that theNa⁺-independentH⁺ extrusion in cultured medullarycells is mediated via H⁺-ATPaseand is upregulated in lethal acidosis. Northern hybridization experiments demonstrated that mRNA levels for the 16- and 31-kDa subunits of H⁺-ATPase remainedunchanged in mutant cells compared with parent cells. We propose thatlethal acid stress results in increased H⁺-ATPase activity in innermedullary collecting duct cells. Upregulation ofH⁺-ATPase could play a protectiverole against cell death in severe intracellular acidosis.

     

cAMP-independent phosphorylation activation of CFTR by G proteins in native human sweat duct

It is generally believed thatcAMP-dependent phosphorylation is the principle mechanism foractivating cystic fibrosis transmembrane conductance regulator (CFTR)Cl channels. However, we showed that activating Gproteins in the sweat duct stimulated CFTR Cl conductance(G_Cl) in the presence of ATP alone without cAMP. The objective of this study was to test whether the G protein stimulation of CFTR G_Cl is independent ofprotein kinase A. We activated G proteins and monitored CFTRG_Cl in basolaterally permeabilized sweat duct.Activating G proteins with guanosine5'-O-(3-thiotriphosphate) (10-100 µM) stimulated CFTRG_Cl in the presence of 5 mM ATP alone withoutcAMP. G protein activation of CFTR G_Cl requiredMg²⁺ and ATP hydrolysis (5'-adenylylimidodiphosphate couldnot substitute for ATP). G protein activation of CFTRG_Cl was 1) sensitive to inhibition bythe kinase inhibitor staurosporine (1 µM), indicating that theactivation process requires phosphorylation; 2) insensitive to the adenylate cyclase (AC) inhibitors 2',5'-dideoxyadenosine (1 mM)and SQ-22536 (100 µM); and 3) independent ofCa²⁺, suggesting that Ca²⁺-dependent proteinkinase C and Ca²⁺/calmodulin-dependent kinase(s) are notinvolved in the activation process. Activating AC with10⁶ M forskolin plus 10⁶ M IBMX (in thepresence of 5 mM ATP) did not activate CFTR, indicating that cAMPcannot accumulate sufficiently to activate CFTR in permeabilized cells.We concluded that heterotrimeric G proteins activate CFTR G_Cl endogenously via a cAMP-independent pathwayin this native absorptive epithelium.

     

Ontogeny and Marginal Growth in the Leaf of Eubrachion ambiguum

Marginal growth in the leaf of Eubrachion ambiguum, a viscaceoushemiparasite, has been investigated. This growth is accomplishedby the marginal meristem comprising the marginal initials aloneas has been described earlier by Hara (1957) in Daphne odora.To the best of the author's knowledge the present communicationis the second report of such a type of marginal growth in thedicotyledons. Phylogenetically, at least in Eubrachion ambiguum, it probablyrepresents a reduced rather than a primitive feature.     

Molecular evolution of bacterial indoleamine 2,3-dioxygenase

Indoleamine 2,3-dioxygenase (IDO) and tryptophan 2,3-dioxygenase (TDO) are tryptophan-degrading enzymes that catalyze the first step in L-Trp catabolism via the kynurenine pathway. In mammals, TDO is mainly expressed in the liver and primarily supplies nicotinamide adenine dinucleotide (NAD⁺). TDO is widely distributed from mammals to bacteria. Active IDO enzymes have been reported only in vertebrates and fungi. In mammals, IDO activity plays a significant role in the immune system while in fungal species, IDO is constitutively expressed and supplies NAD⁺, like mammalian TDO. A search of genomic databases reveals that some bacterial species also have a putative IDO gene. A phylogenetic analysis clustered bacterial IDOs into two groups, group I or group II bacterial IDOs. The catalytic efficiencies of group I bacterial IDOs were very low and they are suspected not to contribute significantly to L-Trp metabolism. The bacterial species bearing the group I bacterial IDO are scattered across a few phyla and no phylogenetically close relationship is observed between them. This suggests that the group I bacterial IDOs might be acquired by horizontal gene transmission that occurred in each lineage independently. In contrast, group II bacterial IDOs showed rather high catalytic efficiency. Particularly, the enzymatic characteristics (K_m, V_max and inhibitor selectivity) of the Gemmatimonas aurantiaca IDO are comparable to those of mammalian IDO1, although comparison of the IDO sequences does not suggest a close evolutionary relationship. In several bacteria, TDO and the kynureninase gene (kynU) are clustered on their chromosome suggesting that these genes could be transcribed in an operon. Interestingly, G. aurantiaca has no TDO, and the IDO is clustered with kynU on its chromosome. Although the G. aurantiaca also has NadA and NadB to synthesize a quinolinic acid (a precursor of NAD⁺) via the aspartate pathway, the high activity of the G. aurantiaca IDO flanking the kynU gene suggests its IDO has a function similar to eukaryotic enzymes.     

Suspension feeding and kleptoparasitism within the genus Trichotropis (Gastropoda: Capulidae)

The marine gastropod Trichotropis cancellata is a facultativekleptoparasite, either suspension feeding or parasitically stealingfood from tube-dwelling polychaete worms. To determine whetherconclusions drawn from long-term studies in the San Juan Islands,Washington, about the relative importance of suspension feedingand kleptoparasitism can be applied generally to T. cancellataacross its biogeographic range, I expanded earlier studies toAlaska and British Columbia. Kleptoparasitism is pervasive throughoutthe range of T. cancellata, occurring with equal frequency throughoutthe areas studied. The average density and size of worm hostsare relatively constant across this range. Snail and worm densitiesare not significantly correlated at the larger scale of site(averaged over nearby sampling locations clustered around acity), but are correlated at the smaller local scale (withina sampling location). Larger worms do not support more snails.The abundance of uninfected worm hosts is usually not limiting,except potentially in some sampling locations in southwest Alaskawhere the use of a novel host (a holothurian) may be the resultof low densities of uninfected worms. Additionally, I documentedthe feeding behaviours of other trichotropid species in theseregions. Trichotropis conica is the second confirmed kleptoparasitewithin the genus Trichotropis, with kleptoparasitism as frequentin this species as in T. cancellata. Like T. cancellata, allsizes observed of T. conica are kleptoparasites. On the otherhand, Trichotropis insignis is an obligate suspension feeder.Further studies are needed to determine exactly how many timesthis behaviour has arisen and been lost in Capulidae and relatedfamilies. (Received 31 May 2007; accepted 19 October 2007)     

Characterization of vectorial chloride transport pathways in the human pancreatic duct adenocarcinoma cell line HPAF

Pancreatic duct cells express a Ca²⁺-activated Cl^- conductance (CaCC), upregulation of which may be beneficial to patients with cystic fibrosis. Here, we report that HPAF, a human pancreatic ductal adenocarcinoma cell line that expresses CaCC, develops into a high-resistance, anion-secreting epithelium. Mucosal ATP (50 µM) caused a fourfold increase in short-circuit current (I_sc), a hyperpolarization of transepithelial potential difference (from -4.9 ± 0.73 to -8.5 ± 0.84 mV), and a fall in resistance to less than one-half of resting values. The effects of ATP were inhibited by mucosal niflumic acid (100 µM), implicating an apical CaCC in the response. RT-PCR indicated expression of hClC-2, hClC-3, and hClC-5, but surprisingly not hCLCA-1 or hCLCA-2. K⁺ channel activity was necessary to maintain the ATP-stimulated I_sc. Using a pharmacological approach, we found evidence for two types of K⁺ channels in the mucosal and serosal membranes of HPAF cells, one activated by chlorzoxazone (500 µM) and sensitive to clotrimazole (30 µM), as well as one blocked by clofilium (100 µM) but not chromanol 293B (5 µM). RT-PCR indicated expression of the Ca²⁺-activated K⁺ channel KCNN4, as well as the acid-sensitive, four transmembrane domain, two pore K⁺ channel, KCNK5 (hTASK-2). Western blot analysis verified the expression of CLC channels, as well as KCNK5. We conclude that HPAF will be a useful model system for studying channels pertinent to anion secretion in human pancreatic duct cells. Ussing chamber; short-circuit current; RT-PCR; immunoblot     

Callus Formation, Plant Regeneration and Clonal Propagation in Vitro of Gynura aurantiaca (Blume) DC.

Methods for culture in vitro of Gynura aurantiaca (Blume) DC.are described. Callus formation from gynura explants was initiallydifficult in spite of the multiple combinations of plant growthregulators assayed. In order to induce high growth rate, incorporationof several organic addenda to a basal medium was necessary,the best of these being coconut milk. Unorganized cell linescould be obtained by subculturing on C medium supplemented with10% coconut milk, and transfers had to be done at short intervals. A morphogenetic cell line without apparent loss in its organogenicpotential through more than 8 months of subculturing was establishedfollowing a sequence of culture media. Methods for rapid and efficient clonal propagation in vitroof this plant species are also reported. The possible utilization of these tissue culture techniquesdeveloped for gynura, a suitable indicator host for Citrus ExocortisViroid, in further studies concerning pathogenesis and replicationof this viroid is discussed. (Received April 22, 1985; Accepted October 11, 1985)