The ultrastructure of M1-a-mediated resistance to powdery mildew infection in barley

1975 ◽  
Vol 53 (22) ◽  
pp. 2589-2597 ◽  
Author(s):  
H. H. Edwards

M1-a-mediated resistance in barley to invasion by the CR3 race of Erysiphe graminis f. sp. hordei does not occur in every host cell with the same speed and severity. In some cells ultrastructural changes within the host cell as a result of resistance will occur within 24 h after inoculation, whereas in other cells these changes may take up to 72 h. In some cells the ultrastructural changes are so drastic that they give the appearance of a hypersensitive death of the host cell, whereas in other cells the changes are very slight. In any case, at the end of these changes the fungus ceases growth. The ultrastructural changes occur in penetrated host epidermal cells as well as non-infected adjacent epidermal and mesophyll cells.The following ultrastructural changes have been observed: (1) an electron-dense material which occurs either free in the vacuole or adhering to the tonoplast (the material is granular or in large clumps); (2) an increased electron density of the host cytoplasm and nucleus; (3) a breakdown of the tonoplast so that the cytoplasmic constituents become dispersed throughout the cell lumen; and (4) the deposition of papillar-like material in areas other than the penetration site. The first three changes take place within the host cell protoplasts and are directly attributable to the gene M1-a. These changes are typical of stress or incompatibility responses and thus M1-a appears to trigger a generalized incompatibility response in the presence of race CR3. The papillar-like material occurs outside the host cell protoplast in the same manner as the papilla and probably is not directly attributable to M1-a.

1990 ◽  
Vol 68 (12) ◽  
pp. 2618-2628 ◽  
Author(s):  
Annerose Heller ◽  
Friedrich Grossmann ◽  
Burkhard Frenzel ◽  
Sigrun Hippe

Light and electron microscopy of barley epidermal cells treated with ethirimol or propiconazole and then inoculated with Erysiphe graminis f. sp. hordei showed the complex reaction of this host–parasite system to fungicides. The completely different biochemical modes of action of the two fungicides were reflected in the ultrastructural changes observed. Specific fungicidal effects could be distinguished from degenerative processes associated with senescence of untreated plants. For ethirimol, the first changes to be observed in the nucleus were blebbing of the outer nuclear membrane, invaginations into the nucleoplasm, and loss of the dark-staining material of nuclear pores. Later on, large areas of the cytoplasm were devoid of ribosomes. Moreover, electron-dense material was found in the perinuclear space and in cisternae of the endoplasmic reticulum. Round bodies, containing electron-dense material of unknown origin, appeared in the cytoplasm. Propiconazole, on the other hand, caused severe malformations of haustoria, host cell wall appositions, and wall thickening. The sheaths surrounding the haustoria were significantly enlarged, and vesicular and multivesicular bodies appeared in the extrahaustorial matrix. In later stages, degenerated haustoria were partially encapsulated by the host cell. Large, rectangular, electron-opaque structures, termed Fibrosinkörper, were observed in secondary hyphae. Both fungicides tested caused swelling of secondary hyphae. Key words: Erysiphe graminis f.sp. hordei, ethirimol, propiconazole, host–parasite system, cytology, electron microscopy.


Parasitology ◽  
1980 ◽  
Vol 80 (1) ◽  
pp. 9-21 ◽  
Author(s):  
M. K. Shaw

SummaryThe epidermis of Diplectanum aequans has, in general, been found to be similar to the epidermis of other monogeneans, consisting of a syncytial outer epidermis and sunken sub-epidermal nucleated regions. However, the epidermis of D. aequans differs from that of other monogeneans in 3 respects. These are, the presence of large areas of granular cytoplasm within the outer epidermis, the presence of myofibres invaginating into the epidermal matrix and, in the posterior regions of the epidermis, the presence of epidermal scales. These scales occur within the epidermal cytoplasm, beneath the outer membrane, and are composed of moderately electron-dense material. Also present beneath the outer membrane in the more anterior regions of the epidermis are small scale-like sclerites of a similar electron density to the epidermal scales.


1986 ◽  
Vol 34 (12) ◽  
pp. 1639-1644 ◽  
Author(s):  
F Kalinec ◽  
J H Calderón ◽  
B Monis

The present report deals with a densitometric study of the ultrastructural images of the urothelial membrane of rats in the following experimental conditions: (1) EFA-deficient (EFAD) rats; (2) EFA-sufficient (EFAS) rats; and (3) EFAD rats that were fed the EFAD diet for 30 weeks and received an EFAS diet for the following 10 weeks (EFAD/S group). On electron micrographs of the transitional epithelium of ureters and urinary bladder of these rats, optical density (OD) profiles of the urothelial unit membrane were recorded and digitized using a computer-controlled microdensitometer with a solid-state self-scanned photodiode array sensor. A Gaussian curve was adopted as a model for the distribution of electron-dense material in each osmiophilic leaflet. Gaussian parameters were used to estimate the thickness of the urothelial membrane and of each osmiophilic leaflet, and the amount of electron-dense material and the maximal electron density present in each leaflet. In EFAS rats, the thick urothelial membrane was asymmetric like that of the normal, resulting from a greater thickness of the outer leaflet and a greater electron density of the cytoplasmic one. In EFAD rats, a loss of the characteristic ultrastructural asymmetry and a decrease of the total thickness of the unit membrane were detected. These changes were partially reversed in the EFAD/S rats.


1976 ◽  
Vol 54 (2) ◽  
pp. 235-244 ◽  
Author(s):  
K. S. Boo ◽  
S. B. McIver

The antenna of female Anopheles stephensi Liston bears three types of sensilla with grooved pegs: those sunken in pits and subtypes A and B of those located on the flagellar surface. The sunken peg sensilla are innervated by four or five neurons with branching dendrites. The dendrites are exposed to the exterior by means of longitudinal clefts at the bases of the grooves in the peg wall. Surrounding the dendrites and extending into the clefts is an extracellular material of medium electron density. Three sheath cells are associated with each sunken peg sensillum.Subtype-A surface peg sensilla are generally similar to the sunken peg sensilla, except that they are located on the antenna) surface and are innervated by two neurons with unbranched dendrites. Subtype-B surface peg sensilla have three or four neurons, the dendrites of which do not branch and are exposed less to the exterior than those in the other peg sensilla because the clefts in the peg wall are smaller and less frequent. Only trace amounts of electron-dense material occur in the clefts of the subtype-B surface peg sensilla.The sunken peg and both subtypes of the surface peg sensilla are probably olfactory receptors.


2018 ◽  
Author(s):  
Mathias Nottensteiner ◽  
Bernd Zechmann ◽  
Christopher McCollum ◽  
Ralph Hückelhoven

ABSTRACTPlant immunity is overcome by pathogens by the means of secreted effectors. Host effector targets might be proteins acting in pathogen defense or serve demands of the pathogen. The barley ROP GTPase HvRACB is involved in entry of the powdery mildew fungusBlumeria graminisf.sp.hordei (Bgh)into barley epidermal cells. We found that HvRACB interacts with theROP-interactive peptide 1 (ROPIP1) that is encoded on the active non-long terminal repeat retroelement Eg-R1 ofBgh. Over-expression of ROPIP1 in barley epidermal cells and host-induced post-transcriptional gene silencing (HIGS) ofROPIP1suggested that ROPIP1 is involved in virulence ofBgh. Bimolecular fluorescence complementation and co-localization supported that ROPIP1 can interact with activated HvRACB in planta. We show that ROPIP1 is expressed byBghon barley and translocated into the cytoplasm of infected barley cells. ROPIP1 is recruited to microtubules upon co-expression of MICROTUBULE ASSOCIATED ROP GTPase ACTIVATING PROTEIN (HvMAGAP1) and can destabilize cortical microtubules.BghROPIP might target HvRACB and manipulate host cell microtubule organization for facilitated host cell entry. Data suggest a possible neo-functionalization of retroelement-derived transcripts for the evolution of a pathogen virulence effector.


1985 ◽  
Vol 117 (1) ◽  
pp. 111-117
Author(s):  
T. D. SCHULTZ ◽  
M. A. RANKIN

Samples of cicindelid cuticle were examined at various stages of adult ecdysis. The multilayered potential reflector was secreted in the initial stages of the moult, verifying that it is not tectocuticle and supporting the contention that it is a form of inner epicuticle. At early stages of ecdysis, the electron-dense layers were visible only when the section was post-stained. During post-ecdysial colour development, the dense layer increased in inherent electron density. Concurrently, the reflector increased in refractive index and the interference coloration increased in intensity and wavelength of maximum reflectance. Black pigment was also deposited simultaneously within the outer portion of the cuticle. It is proposed that electron-dense material was deposited in situ within the inner epicuticle after ecdysis, thereby increasing the wavelength and reflectance of interference colour.


Development ◽  
1978 ◽  
Vol 46 (1) ◽  
pp. 75-87
Author(s):  
E. E. Ball ◽  
A. N. Cowan

The cuticle in the tympanal area of immature crickets, Teleogryllus commodus (Walker), is ultrastructurally indistinguishable from that elsewhere on the prothoracic leg. It is only in the pharate adult that changes associated with development of the tympana first appear. In pharate adults and adults the external layer of the tympana consists of a layer of electrondense material overlying a layer where the electron-dense material is interspersed with cuticle in which the bundles of microfibrils are coarser and more loosely arranged than elsewhere in the leg. The innermost portion of the tympana consists of this same type of cuticle without the electron-dense material. Associated with the appearance of the electron-dense material in the tympana of the pharate adult is a change in the toluidine blue staining properties from blue to deep purple. The reaction of the tympana in acid and base is consistent with their being composed of chitin. There are no major deposits of resilin in the tympana. In the first few days following the imaginal ecdysis the posterior tympanum and underlying trachea come into tight apposition due to the withdrawal of the epidermal cells. The epidermal cells do not withdraw from beneath the anterior tympanum. The surrounding non-tympanal cuticle continues to thicken for several weeks with the result that in the mature adult the posterior tympanum serves as an acoustic window in the thick cuticle of the leg. The functional significance of the anterior tympanum has not been established.


Author(s):  
J. R. Ruby ◽  
R. F. Dyer ◽  
R. G. Skalko ◽  
R. F. Gasser ◽  
E. P. Volpe

An electron microscope examination of fetal ovaries has revealed that developing germ cells are connected by intercellular bridges. In this investigation several species have been studied including human, mouse, chicken, and tadpole (Rana pipiens). These studies demonstrate that intercellular connections are similar in morphology regardless of the species.Basically, all bridges are characterized by a band of electron-dense material on the cytoplasmic side of the tri-laminar membrane surrounding the connection (Fig.l). This membrane is continuous with the plasma membrane of the conjoined cells. The dense material, however, never extends beyond the limits of the bridge. Variations in the configuration of intercellular connections were noted in all ovaries studied. However, the bridges in each individual species usually exhibits one structural characteristic seldom found in the others. For example, bridges in the human ovary very often have large blebs projecting from the lateral borders whereas the sides of the connections in the mouse gonad merely demonstrate a slight convexity.


1992 ◽  
Vol 70 (1) ◽  
pp. 58-72 ◽  
Author(s):  
Jeffrey G. Duckett ◽  
Roberto Ligrone

The ventral epidermal cells of the photosynthetic, surface-living gametophytes of Lycopodium cernuum, collected from moist shaded banks in Peninsular Malaysia, contain an aseptate fungus. In some cells the hyphae are thick walled and form coils encapsulated by a thin layer of host wall material. In others the fungus is thin walled and shows limited differentiation into larger trunk hyphae and arbuscules. The adjacent host cytoplasm, separated from the fungus by a granular interfacial matrix, contains numerous chloroplasts, mitochondria, and microtubules. The hyphae contact the substratum via the ventral walls of the epidermal cells and the rhizoids are free from infection. In the protocorm and root nodules, aseptate hyphae initially colonize mucilage-filled schizogenous intercellular spaces. Subsequent invasion of the host cells is associated with the development of massive overgrowths of host wall material. The fungal associations in L. cernuum share a mixture of attributes otherwise found in different angiosperm mycorrhizae and in mycotrophic relationships in liverworts. Wall ingrowths are present in both the gametophyte and sporophyte cells in the placenta of L. cernuum. The very limited development of the placenta, compared with L. appressum, certain bryophytes and ferns, the diminutive size, and early senescence of the gametophytes of L. cernuum are all linked to the presence of the protocorm. This massive absorptive organ, homologous to a foot, in terms of its position in sporophyte ontogeny, but external to the parent gametophyte, derives its nutrition partly from photosynthesis and partly from its fungal endophyte. Key words: chloroplasts, Lycopodium, mycorrhiza, pteridophytes, root nodules, symbiosis, transfer cells.


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