The vacuolar ATPase ofNeurospora crassa

The filamentous fungusNeurospora crassa has many small vacuoles which, like mammalian lysosomes, contain hydrolytic enzymes. They also store large amounts of phosphate and basic amino acids. To generate an acidic interior and to drive the transport of small molecules, the vacuolar membranes are densely studded with a proton-pumping ATPase. The vacuolar ATPase is a large enzyme, composed of 8–10 subunits. These subunits are arranged into two sectors, a complex of peripheral subunits called V₁ and an integral membrane complex called V₀. Genes encoding three of the subunits have been isolated.vma-1 andvma-2 encode polypeptides homologous to the and subunits of F-type ATPases. These subunits appear to contain the sites of ATP binding and hydrolysis.vma-3 encodes a highly hydrophobic polypeptide homologous to the proteolipid subunit of vacuolar ATPases from other organisms. This subunit may form part of the proton-containing pathway through the membrane. We have examined the structures of the genes and attempted to inactivate them.     

Slime a plasmodioid variant ofNeurospora crassa

The slime variant of Neurospora is unique among the higher Fungi in growing on an agar surface by plasmodium-like outflows which are devoid of cell walls, and in which cells from older parts of an agar colony, and those in liquid culture, have very deficient cell walls. Heterocaryon studies indicate that the nucleus determines the slime phenotype. Genetic studies show that three independently inherited characters are essential to but insufficient for the slime phenotype. Some, but not all isolates with all three characteristics give rise to vegetatively derived isolates with stable slime phenotypes.Supported in part by grant G-6174 from the National Science Foundation, and in part by grant GM-06965 from the National Institutes of Health, U.S. Public Health Service.     

Nickel transport in nickel-resistant strains ofNeurospora crassa

Transport of Ni²⁺ has been studied in three Ni²⁺-resistant strains ofNeurospora crassa (Ni^R1, Ni^R3) and Ni^R3) and in the parent wild strainN. crassa Em 5297a. Several strainspecific differences have been found. Rates of Ni²⁺ uptake were Ni^R2>Ni^R1>Em>>Ni^R3. While K_m for Ni²⁺ uptake was similar, V_max values were sharply different, with Ni^R3 having the lowest value. Observed uptake was entirely due to transport into the intracellular phase. Transport was strongly pH dependent only in Em, Ni^R1, and Ni^R2, which had a pH optimum at 4; optimum was at pH 5 for Ni^R3. Mg²⁺ was powerfully inhibitory to Ni²⁺ uptake in Ni^R1 and Ni^R2, but was less efficient in Ni^R3; in contrast, Mn²⁺ was most inhibitory in Ni^R3. It has been suggested that Ni²⁺ resistance in Ni^R3 is specifically due to lowered levels of the Ni²⁺ transport system herein.     

Metal ion influence on the growth inhibition ofNeurospora crassa by bacitracin

The growth-inhibitory activity of bacitracin onNeurospora crassa is dependent on the source of nitrogen and phosphate, as well as the presence of certain divalent metal ions in the medium. Whereas supplementation of manganese, calcium, and magnesium resulted in the mitigation of the growth inhibition by bacitracin, supplemental copper, in contrast, potentiated it more than 30-fold over controls, as evidenced by 50% growth-inhibitory (I₅₀) values. Bacitracin interfered with the transport of metal ions, as observed with an altered contents of Mn²⁺, Cu²⁺, Na⁺, and K⁺ in bacitracin ±Cu²⁺-treated cultures vs. controls. The decreased K⁺ content in bacitracin ±Cu²⁺-treated cultures indicated possible membrane damage as the mechanism of action. Alterations in amino acid pool size and total nitrogen content induced by bacitracin are secondary effects as a consequence of the loss of membrane permeability.     

Cobalt transport in nickel-resistant strains ofNeurospora crassa

Uptake of Co²⁺ by three nickel-resistant strains (Ni^R1, Ni^R2, and Ni^R3) ofNeurospora crassa that differed in resistance to Co²⁺ has been studied. Uptake was linear with Co²⁺ concentration (up to 1 mM), with time (up to 6 h), and with pH between 3 and 6. Uptake rates were in the order Ni^R2>Ni^R1>Ni^R3. In all strains, there was gradual increase in Co²⁺ uptake between 10° and 28°C, with a much sharper increase between 28° and 40°C. Metabolic inhibitors decreased Co²⁺ uptake partially in all strains, except for KF in Ni^R3. About 50–80 g Co²⁺/100 mg dry weight was surface bound. Ni²⁺, Zn²⁺, and Mn²⁺ competed with Co²⁺, the effects being strain specific. Mg²⁺ inhibited Co²⁺ uptake in all strains with preformed mycelia. In Ni^R1 and Ni^R2 only with young mycelia (40 h old) was Mg²⁺ inhibitory to Co²⁺ uptake,during growth in the presence of Co²⁺. The results suggested the presence of two transport systems for Co²⁺ in Ni^R1 and Ni^R2, only one of which was sensitive to Mg²⁺; in contrast, Ni^R3 had a single system, which was sensitive to Mg²⁺.     

Cobalt transport in a cobalt-resistant strain ofNeurospora crassa

Uptake of Co²⁺ by cobalt-resistant strain is dependent on Co²⁺ concentration in the medium and is linear with time. The uptake is unaffected by metabolic inhibitors and decreased at low pH values. The uptake is independent of temperature in the range 0–40‡ C. The transport system is a passive diffusion process, unlike in the parent wild type strain where it is energy-dependent. It is possible that Mg²⁺ transport system is not involved in Co²⁺ transport in this strain, since the Co²⁺ uptake is not suppressed by Mg²⁺ as in the parent strain.     

Studies on copper toxicity in nickel-resistant strains ofNeurospora crassa

Copper toxicity has been studied in three nickel-resistant strains ofNeurospora crassa (Ni^R1, Ni^R2, and Ni^R3). Ni^R1 and Ni^R2, but not Ni^R3, were two-to threefold more sensitive than the parent wild strain (N. crassa EM 5297a) to Cu²⁺ on a normal N medium. On a nitrate N medium, Cu²⁺ was 16-fold more toxic to Ni^R3 because of reduced synthesis of nitrite reductase; Ni^R1 and Ni^R2 were only fivefold more sensitive to Cu²⁺, and nitrite reductase synthesis was unaffected. Mn²⁺ reversed Cu²⁺ toxicity on normal N medium only, in all strains. Fe³⁺ counteracted Cu²⁺ toxicity on nitrate N medium also. It was shown that Cu²⁺ affected Fe³⁺ utilization for nitrite reductase synthesis in Ni^R3 only and that in these Ni²⁺-resistant strains, Fe³⁺ antagonized effects of Cu²⁺, but not of other toxic metal ions.     

Crossing-over across the centromere in the mating-type chromosome ofNeurospora crassa

The frequency of crossing-over in the two short regions on opposite arms, adjacent to the centromere of the mating-type chromosome ofNeurospora crassa is controlled, independently in each arm, by at least two genes with equal and additive effect. These genes segregate on inbreeding and cause great variability in both the frequency of recombination and the frequency of second-division segregation of loci situated within these regions. Recombination values between loci situated beyond these sensitive regions is not affected; the relative increase or decrease in their centromere distances may be attributed to change in the recombination frequency about the centromere only.     

Transcellular ion currents and extension ofNeurospora crassa hyphae

Summary Hyphae ofNeurospora crassa, like many other tipgrowing organisms, drive endogenous electric currents through themselves such that positive charges flow into the apical region and exit from the trunk. In order to identify the ions that carry the current, the complete growth medium was replaced by media lacking various constituents. Omission of K⁺ or of phosphate diminished the zone of inward current, effectively shifting the current pattern towards the apex. Omission of glucose markedly reduced both inward and outward currents; addition of sodium azide virtually abolished the flow of electric current. Growing hyphae also generate a longitudinal pH gradient: the medium surrounding the apex is slightly more alkaline than the bulk phase, while medium adjacent to the trunk turns acid. The results suggest thatNeurospora hyphae generate a proton current; protons are expelled distally by the H⁺-ATPase and return into the apical region by a number of pathways, including the symport of protons with phosphate and potassium ions. Calcium influx may also contribute to the electric current that enters the apical region. There seems to be no simple obligatory linkage between the intensity of the transcellular electric current and the rate of hyphal extension. Calcium ions, however, are required in micromolar concentrations for extensions and morphogenesis of hyphal tips.     

Freeze-etch and thin section studies ofNeurospora crassa ascospores

Summary Mature, dormant ascospores derived from crosses of wild type stocks of the fungusNeurospora crassa were studied using both thin section and freeze-etch techniques for electron microscopy. The spore wall is composed of three major layers with, perhaps, a fourth distinct layer covering these layers. The spore contains several nuclei, many discrete mitochondria, lipid bodies, vacuoles and small pieces of endoplasmic reticulum. Freeze-etch fracture faces of several membranes are described in this paper. Included is a diagram illustrating various fracture faces and surfaces seen following freeze-etching. The thin section results are less than satisfactory but serve to generally confirm the freeze-etch observations and suggest that further work could lead to the development of techniques which will result in high quality thin sections of ascospores.     

Permeabilization ofNeurospora crassa hyphae with toluene-ethanol and filipin

Young hyphae ofNeurospora crassa were made permeable to UDP-glucose and trypan blue by treatment with toluene-ethanol and filipin. Less than 2% of treated cells survived treatment with 8% and 16% toluene-ethanol, while 25% survived treatment with 4% toluene-ethanol. Similarly, 98% of treated cells were killed by treatment with 16 g/ml filipin. Electron microscopy revealed that toluene-ethanol-treated cells lost pieces of plasma membrane and contained a number of vacuole-like structures; filipin-treated cells were less affected. Both filipin- and toluene-ethanol-treated cells were able to incorporate UDP-glucose into insoluble material (likely glycogen and glucan).     

Preparation of highly purified mitochondria ofNeurospora crassa on a Percoll gradient

Mitochondria isolated from Neurospora crassa were purified by centrifugation in a Percoll density gradient. Enzyme activities and cytochrome differential spectra revealed a high purity of the mitochondria. As compared with a crude mitochondrial fraction the purified mitochondria exhibited a high respiratory activity and a fine ADP/O ratio. Electrophoresis of nucleic acids demonstrated the absence of cytoplasmic rRNA.     

A study of the messenger RNA encoding pyruvate kinase ofNeurospora crassa

InNeurospora crassa, there is a single pyruvate kinase (PK) consisting of four identical subunits of 60k daltons. Northern and dot blot hybridization studies, using most of the yeast pyruvate kinase gene as a probe, suggest the presence of two distinct mRNA species for pyruvate kinase, separable on the basis of the length of their polyadenylated tails, by oligo(dT)cellulose chromatography. These messages are present in polysomes, immuno-precipitated by anti-PK antibodies, indicating probable translation in vivo. Fractions containing both messages were translatedin vitro in the heterologous systems as well as in a homologousN. crassa lysate, the newly-synthesized PK being detected by immunoadsorption. Protection studies using S1-nuclease suggest no major structural differences in the 5-untranslated and most of the coding regions of the two messages.     

Conidiation ofNeurospora crassa in submerged culture without mycelial phase

Summary Conidia ofNeurospora crassa shaken in liquid cultures at 46°C for 15 h and then shifted-down to 25°C germinate directly into conidiophores producing new conidia (macroconidia).     

In vivo absorption spectra ofNeurospora crassa white collar photomutants

White collar (wc) mutants ofNeurospora crassa, which lack several responses to blue light, did not have altered absorption spectra when compared to a control strain. We conclude either that thewc mutants do not lack photoreceptor pigments or alternatively that the photoreceptors are present at levels too low to detect. The results show that carotenoids can be genetically reduced to a level at which they should not interfere with spectrophotometric attempts to detect the blue light receptors.