Antibacterial activity of α-terpineol may induce morphostructural alterations in Escherichia coli

The antibacterial effect of α-terpineol from Cinnamomum longepaniculatum (Gamble) N. Chao leaf essential oils were studied with special reference to the mechanism of inhibiting the standard strain of Escherichia coli (CMCC (B) 44102) growth at ultrastructural level. Minimal inhibitory concentration (MIC) and minimal bactericidal concentration (MBC) and time-kill curves of α-terpineol were determined; Escherichia coli was treated with α-terpineol and observed under a transmission electron microscope. The MIC and MBC values of α-terpineol were all 0.78 µL/mL, and time-kill curves showed the concentration-dependent. Under the transmission electron microscopy (TEM), Escherichia coli exposed to MIC levels of α-terpineol exhibited decreased cell size and irregular cell shape, cell wall and cell membrane were ruptured, nucleus cytoplasm was reduced and nuclear area gathered aside. Results suggest that α-terpineol has excellent antibacterial activity and could induce morphological changes of Escherichia coli.

Subcellular localization of cadmium in the root cells of Allium cepa by electron energy loss spectroscopy and cytochemistry.

The ultrastructural investigation of the root cells of Allium cepa L. exposed to 1 mM and 10 mM cadmium (Cd) for 48 and 72 h was carried out. The results indicated that Cd induced several obvious ultrastructural changes such as increased vacuolation, condensed cytoplasm with increased density of the matrix, reduction of mitochondrial cristae, severe plasmolysis and highly condensed nuclear chromatin. Electron dense granules appeared between the cell wall and plasmalemma. In vacuoles, electron dense granules encircled by the membrane were aggregated and formed into larger precipitates, which increase in number and volume as a consequence of excessive Cd exposure. Data from electron energy loss spectroscopy (EELS) confirmed that these granules contained Cd and showed that significantly higher level of Cd in vacuoles existed in the vacuolar precipitates of meristematic or cortical parenchyma cells of the differentiating and mature roots treated with 1 mM and 10 mM Cd. High levels of Cd were also observed in the crowded electron dense granules of nucleoli. However, no Cd was found in cell walls or in cells of the vascular cylinder. A positive Gomori-Swift reaction showed that small metallic silver

Fine structural study of the red seaweed Gymnogongrus torulosus (Phyllophoraceae, Rhodophyta)

The present study analyzed several characters of the red seaweed Gymnogongrus torulosus, such as cellular structure of the thallus, cuticle, pit plug and cell wall ultrastructure, and morphology of some organelles like plastids, Golgi bodies and mitochondria. Also, anomalous chloroplasts with thylakoid disorganization were found in medullary cells. The significance of this thylakoid disposition is still unclear. This is one of the first studies focused on the fine structure of a red alga recorded in Argentina.

Effect of sugars on the association between cowpea vicilin (7S storage proteins) and fungal cells

Vicilins (7S storage proteins) found in various legume seeds have been previously shown to interfere with the germination of spores or conidia of phytopathogenic fungi and inhibit yeast growth and glucose stimulated acidification of the medium by yeast cells. In the present work vicilins from cowpea (Vigna unguiculata) seeds were added to the growth medium of Saccharomyces cerevisiae cells and Fusarium oxysporum conidia. Helix pomatia lectin, wheat germ agglutinin and Ulex europaeus lectin were used to identify differences in the binding of the vicilins to the surface of cells of S. cerevisiae and F. oxysporum treated with this protein. After the growth period, the material in suspension (yeast cells) was centrifuged and the final pellet was also treated with different sugar (glucose, sucrose, glucosamine, N-acetyl-glucosamine) concentrations and 0.1 M HCl for extraction of vicilins associated to chitinous structures present in yeast cells. Our results showed that vicilin sub-units were present in the different sugar extracts of yeast cells pretreated with the vicilins and these proteins were eluted by 0.5 M solutions of sugars in the following order of efficiency of elution: N-acetyl-glucosamine, sucrose/glucose and glucosamine.

Distribution of pectins in the pollen apertures of Oenothera hookeri: velans ster/+ster

Cell wall pectins are some of the most complex biopolymers known, and yet their functions remain largely mysterious. The aim of this paper was to deepen the study of the spatial pattern of pectin distribution in the aperture of Oenothera hookeri.velans ster/+ster fertile pollen. We used "in situ" immunocytochemical techniques at electron microscopy, involving monoclonal antibodies JIM5 and JIM7 directed against pectin epitopes in fertile pollen grains of Oenothera hookeri.velans ster/+ster. The same region was also analyzed by classical cytochemistry for polysaccharide detection. Immunogold labelling at the JIM7 epitope showed only in mature pollen labelling mainly located at the intine endo-aperture region. Cytoplasmic structures near the plasma membrane of the vegetative cell showed no labelling gold grains. In the same pollen stge the labelling at the JIM5 epitope was mostly confined to a layer located in the limit between the endexine and the ektexine at the level of the border of the oncus. Some tubuli at the base of the ektexine showed also an accumulation of gold particles. No JIM5 label was demonstrated in the aperture chamber and either in any cytoplasmic structure of the pollen grains. The immunocytochemical technique, when compared with the traditional methods for non-cellulose polysaccharide cytochemistry is fare more sensitive and allows the univocal determination of temporal and spatial location of pectins recognized by the JIM7 and JIM5 MAbs.

Congo red effect on cyst viability and cell wall structure of encysting entamoeba invadens

Background. The cell wall of Entamoeba invadens cysts is composed of chitin microfibrils as the main structural component. It has been demonstrated in yeast that the chitin cell wall assembly is altered by dyes such as Congo red (CR) and Calcofluor. Methods. The purpose of this work was to study the cell wall assambly under the effect of CR dye on encysting E. invadens by means of light and electron microscopy, after the ammebas were subjected to the effect of 100-2,000 µg CR/mL. Experiments were performed either in BI-S-33 or in mLG media. Results. Trophozoit growth was not inhibited by 100-1,000 µg/mL CR after 8 days of incubation in BI-S-33 medium. However, low levels of growth were observed with 2,000 µg/mL of dye. No significant differences in morphologically viable (hyaline) cyst production occurred after 24-48 hm when 100 µg CR/mL was used, while the highest concentration of CR (2,000 µg/mL) resulted in a significant decrease of hyaline cyst yield; dead cysts prevailed in cultures, particularly at 72 h of CR treatment. Differentiation of amebas incubated in the presence of 500-2,000 µg/mL CR produced abnormal chitin deposits, rendering irregulary thick or double cell walls, as shown by transmission and scanning electron microscopy. Cyst cultures obtained under 100 µg/mL CR produced as many trophozoites as did the control when they were incubated in BI-S-33, but only low numbers of trophozoites were found in culture cysts obtained under higher CR doses. Conclusion. Our results suggest that CR affects E. invadens encystment, alters the cell wall formation, and also affects the cyst viability

Extraction and characterization of proteins from cell walls of two strains of paracoccidioides brasiliensis

En el presente trabajo se analizaron las proteínas de la pared celular de 2 cepas de paracoccidioides brasiliensis en fase levaduriforme (PbHC-PE y Pb 18). Las proteínas fueron extraidas por tres difrentes métodos y estudiadas por electroféresis SDS-PAGE. Los resultados de los perfiles de las dos cepas fueron diferentes, permitiendo la posibilidad de su uso como marcadores quimiotaxonómicos. Se observó una secreción transitoria de la proteína gp 43 a través de la pared celular de las cepas de p. brasiliensis.

Cell wall deficiency in slime strains of Neurospora crassa: osmotic inhibition of cell wall synthesis and Beta-D-glucan synthase activity

1. The RCP-3 S/H mutant of Neurospora crassa was obtained by vegetative selection in medium of high osmolarity of a mycelial form an fz, sg, os-1 ("smile"-like) segregant. The mutant exhibits spheroplast-hyphal dimorphism conditioned by the osmolarity of the culture medium (pietro et al. (1990). Journal of General Microbiology, 136: 121-129). The carbohydrate composition of the cell wall of the mutant was different from that of the wild type in the absence of an alkalisoluble galactosaminoglycan polymer. Furthermore the mutant cell wall had a somewhat lower content of ß-glucan relative to that of chitin. 2. Increasing concentrations of sorbitol in the culture medium of the mutant inhibited by 10-fold the formation of cell wall relative to toal biomass. The cell wall of the mutant cultured in the presence of sorbitol lacked mannose-and galactose-containing polymers, and also showed progressively lower amounts of ß-glucan relative to chitin. 3. The activity of membrane-bound (1-3)-ß-D-glucan synthase from the mutant grown in the absence of sorbitol shared several properties with the wil type enzyme (i.e., Km app, Vmax, stability at 30ºC, activation by GTPyS, and dissociability by treatment with NaCl and Tergitol NP-40 into a membrane-bound catalytic center and GTP-binding activating protein). On the other hand, the enzyme from the mutant but not that from the wild type was inactivated by about 15 per cent by treatment with NaCl and detergent. 4. At high concentrations of sorbitol (1.0M) the RCP-3 S/H mutant exclusively produced spheroplasts devoid of (1-3)-ß-D-glucan synthase activity. The defect was at the level of the membrane-bound catalytic center. The activity of the GTP-binding activating factor was apparently normal in these cells. 5. These results suggest that the definitive loss of cell wall in the N. crassa "slime" RCP-3 S/H mutant was due to a defect in (1-3)-ß-D-glucan synthase activity which wass exaggerated in the presence of high osmolyte concentrations

Aspectos ultraestruturais da parede celular do Paracoccidioides brasiliensis, nas fases micelial e leveduriforme / Ultrastructural aspects of Paracoccidioides brasiliensis cell wall inthe mycelial and yeast phases

A parede celular de uma cêpa de Paracoccidioides brasiliensis, recém isolada de paciente portador de paracoccidioidomicose, foi estudada ultraestruturalmente, empregando-se a microscopia eletrônica de transmissäo e de varredura. Na fase micelial, as observaçöes com o microscópio eletrônico de transmissäo demonstram que a parede celular é composta por duas camadas eletronicamente distintas, sendo que a mais externa é de difícil visualizaçäo e composta possivelmente por delgadas fibrilas de beta-1,3-glucana. Esta camada relaciona-se com outra intermediária, de natureza quitinosa que sobrepoe-se à membrana plasmática. As células quando observadas em microscópio de varredura, apresentam a superfície lisa com anelaçöes septais e formando ocasionalmente clamidoconídeos sub-globosos. A parede celular da fase leveduriforme quando observada em microscopia de transmissäo, apresenta-se recoberta externamente por uma camada nitidamente fibrilar que desaparece quando as células såo tratadas por soluçöes alcalinas. Presume-se que estas fibrilas sejam compostas principalmente por um polisacarídeo, a alfa-1,3-glucana, responsável pela virulência do Paracoccidioides brasiliensis. Esta camada é intensamente corada por um corante monocatiônico, a safranina 0, podendo-se observar que as fibrilas superficiais extendem-se à distância da parede celular. A mesma fase quando preparada para microscopia de varredura pelo método do ponto crítico, apresenta-se recoberta por uma rede microfibrilar de textura grosseira, também álcali-solúvel, apresentando constantemente células de formato esférico ou sub-globoso. Uma outra cêpa do fungo, isolada e mantida em cultivo por 13 anos, apresenta uma rede microfibrilar superficial de textura diversa à da cêpa de isolamento recente e também uma tendência a desenvolver formas alongadas de brotamento, sugerindo uma alteraçäo constitucional da camada de alfa-1,3-glucana e possivelmente uma diminuiçäo da virulência sem a perda da antigenicidade. Säo discutidas as funçoes da alfa-1,3-glucana na patogenia da paracoccidioidomicose, especulando-se sobre a funçäo protetora deste polissacarídeo contra a destruiçäo pelas células do sistema imune