Mutational Activation of a G{alpha}i Causes Uncontrolled Proliferation of Aerial Hyphae and Increased Sensitivity to Heat and Oxidative Stress in Neurospora crassa

Mutational Activation of a G ${alpha}$ _i Causes Uncontrolled Proliferation of Aerial Hyphae and Increased Sensitivity to Heat and Oxidative Stress in Neurospora crassa

Qi Yang^a and Katherine A. Borkovich^a
^a Department of Microbiology and Molecular Genetics, University of Texas, Houston Medical School, Houston, Texas 77030

Corresponding author: Katherine A. Borkovich, Department of Microbiology and Molecular Genetics, University of Texas, Houston Medical School, 6431 Fannin St., Ste. JFB 1.765, Houston, TX 77030., borkovic{at}utmmg.med.uth.tmc.edu (E-mail)

Communicating editor: R. H. DAVIS

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Heterotrimeric G proteins, consisting of ${alpha}$ , ß, and ${gamma}$ subunits,transduce environmental signals through coupling to plasma membrane-localizedreceptors. We previously reported that the filamentous fungusNeurospora crassa possesses a G ${alpha}$ protein, GNA-1, that is a memberof the G ${alpha}$ _i superfamily. Deletion of gna-1 leads to defects inapical extension, differentiation of asexual spores, sensitivityto hyperosmotic media, and female fertility. In addition, ${Delta}$ gna-1strains have lower intracellular cAMP levels under conditionsthat promote morphological abnormalities. To further definethe function of GNA-1 in signal transduction in N. crassa, weexamined properties of strains with mutationally activated gna-1alleles (R178C or Q204L) as the only source of GNA-1 protein.These mutations are predicted to inhibit the GTPase activityof GNA-1 and lead to constitutive signaling. In the sexual cycle,gna-1^R178C and gna-1^Q204L strains are female-fertile, but producefewer and larger perithecia than wild type. During asexual development,gna-1^R178C and gna-1^Q204L strains elaborate abundant, long aerialhyphae, produce less conidia, and possess lower levels of carotenoidpigments in comparison to wild-type controls. Furthermore, gna-1^R178Cand gna-1^Q204L strains are more sensitive to heat shock andexposure to hydrogen peroxide than wild-type strains, while ${Delta}$ gna-1 mutants are more resistant. In contrast to ${Delta}$ gna-1 mutants,gna-1^R178C and gna-1^Q204L strains have higher steady-state levelsof cAMP than wild type. The results suggest that GNA-1 possessesseveral Gß ${gamma}$ -independent functions in N. crassa. We proposethat GNA-1 mediates signal transduction pathway(s) that regulateaerial hyphae development and sensitivity to heat and oxidativestresses, possibly through modulation of cAMP levels.

HETEROTRIMERIC G proteins ( ${alpha}$ ß ${gamma}$ ) are central components ofsignaling pathways in eukaryotic cells (BIRNBAUMER 1992 ). Theheterotrimer is coupled to seven-helix plasma membrane receptors,which sense extracellular ligands. Ligand binding to the receptorcauses GDP-GTP exchange on the G ${alpha}$ subunit, leading to dissociationof the heterotrimer into G ${alpha}$ and Gß ${gamma}$ subunits. Dependingon the system, either G ${alpha}$ or Gß ${gamma}$ can function to regulatedownstream effector proteins.

Hydrolysis of GTP to GDP by the G ${alpha}$ subunit leads to inactivationof signaling and reassociation of the G ${alpha}$ with Gß ${gamma}$ . G ${alpha}$ mutationsresulting in defective GTPase activity have been identifiedthat are dominant in trans and lead to constitutive signaling(JOHNSON et al. 1994 ). In mammals, mutation of either a conservedarginine (201 in G ${alpha}$ _s or 178 in G ${alpha}$ _i1) or a glutamine (227 in G ${alpha}$ _sor 204 in G ${alpha}$ _i1) leads to activation of G ${alpha}$ proteins (FREISSMUTHand GILMAN 1989 ; GRAZIANO and GILMAN 1989 ; COLEMAN et al.1994 ). Mutation of these residues in G ${alpha}$ _s causes ~100-fold lowerGTPase activity in vitro (FREISSMUTH and GILMAN 1989 ; GRAZIANOand GILMAN 1989 ). The slower rate of GTP hydrolysis resultsin constitutive activation of G ${alpha}$ _s due to higher GTP occupancy(FREISSMUTH and GILMAN 1989 ; GRAZIANO and GILMAN 1989 ). Comparisonof crystal structures for wild-type and mutant forms of theG ${alpha}$ _i1 protein demonstrates that the R178 and Q204 residues arecritical for stabilization of the transition state during GTPhydrolysis (COLEMAN et al. 1994 ). Studies using mutant G ${alpha}$ _i2alleles demonstrated that Q205L had higher transformation potentialthan R179C; this result was predicted based on the greater stabilityof the Q205L protein (HUDSON et al. 1981 ; GUPTA et al. 1992).

Phenotypes observed in cells with GTPase-deficient G ${alpha}$ allelescan result from the action of the activated G ${alpha}$ or the free ß ${gamma}$ dimer on effector pathways (BIRNBAUMER 1992 ). An example inwhich free ß ${gamma}$ is the active unit is the mating/pheromoneresponse pathway in the yeast Saccharomyces cerevisiae. In thissystem, the Ste4p/Ste18p ß ${gamma}$ heterodimer positively regulatesa mitogen-activated protein (MAP) kinase pathway, leading tocell-cycle arrest and mating (reviewed by BORKOVICH 1996 ).The function of the Gpa1p G ${alpha}$ is to tether ß ${gamma}$ , renderingit inactive; thus, strains with null or GTPase-deficient gpa1G ${alpha}$ alleles exhibit similar cell-cycle arrest phenotypes (reviewedby KURJAN 1992 ).

Neurospora crassa GNA-1 is a member of the G ${alpha}$ _i superfamily, basedon amino acid sequence identity and its ability to serve asa substrate for pertussis toxin (TURNER and BORKOVICH 1993 ; IVEY et al. 1996 ). ${Delta}$ gna-1 strains are defective in severalcellular processes, including apical extension on solid mediumwith or without hyperosmotic agents, aerial hyphae development,and female fertility (IVEY et al. 1996 ). Furthermore, ${Delta}$ gna-1strains have reduced intracellular cAMP levels under conditionsthat promote morphological abnormalities (D. IVEY, Q. YANG andK. BORKOVICH, unpublished results).

cAMP is implicated in regulation of several processes in N.crassa. Carotenoid pigment accumulation is negatively correlatedwith the steady-state level of cAMP (KRITSKY et al. 1982 ),exogenous cAMP reduces carotenoid synthesis (HARDING 1973 ),and lower cAMP levels trigger derepression of carotenoid genetranscription (reviewed by BRAMLEY and MACKENZIE 1988 ). Mutationof the regulatory subunit of cAMP-dependent protein kinase (PKA)causes loss of growth polarity (BRUNO et al. 1996 ), while hyphalelongation is regulated by a kinase exhibiting homology to thecatalytic subunit of PKAs (YARDEN et al. 1992 ). Furthermore,analysis of an adenylyl cyclase-deficient mutant (cr-1) hasprovided evidence that cAMP plays a positive regulatory roleduring basal hyphae growth and in aerial hyphae formation (TERENZIet al. 1974 ). Studies using ${Delta}$ gna-1 strains also support a positiverole for cAMP in hyphal growth and aerial hyphae formation (D.IVEY, Q. YANG and K. BORKOVICH, unpublished results).

cAMP has been linked to responses to heat and oxidative stressin several fungal species. In S. cerevisiae and N. crassa, mutationsin adenylyl cyclase lead to increased resistance to lethal heattreatment. This phenomenon results from a decrease in cAMP levelsand subsequent lower PKA activity (SHIN et al. 1987 ; CRUZet al. 1988 ). S. cerevisiae bcy1 mutants are deficient in theregulatory subunit of PKA and contain a constitutively activecatalytic PKA subunit; these strains are more sensitive to heat(SHIN et al. 1987 ). Available evidence suggests that cAMP controlof heat sensitivity and heat shock protein synthesis is largelyindependent of heat shock promoter elements (HSEs) and the heatshock transcription factor Hsf1p (MAGER and DE KRUIJFF 1995). Recently, a cAMP-regulated stress responsive promoter element,or STRE, has been identified in S. cerevisiae (MARCHLER et al.1993 ). This sequence is implicated in regulation of gene expressionby a variety of environmental stresses, including heat and oxidants.However, regulation by STRE alone cannot explain the observedlevels of expression of all stress-regulated genes. Hence, ithas been postulated that both general control by STRE and specificcontrol by other elements is required for appropriate regulationof genes in response to environmental stress (MAGER and DE KRUIJFF1995 ).

In this study, we characterize the properties of N. crassa strainswith null, wild-type, gna-1^Q204L, or gna-1^R178C GTPase-deficientalleles as the only source of GNA-1 protein. We analyze levelsof G protein subunits and report phenotypes for the strainsduring both vegetative and sexual phases of the life cycle.We also quantitate intracellular cAMP and carotenoid levels,and measure sensitivity to heat and hydrogen peroxide in thevarious strains. We demonstrate a Gß ${gamma}$ -independent rolefor GNA-1 during several processes in N. crassa. We furthershow that in many cases the extent of the observed phenotypescan be correlated with the predicted GTP-occupancy of GNA-1.

MATERIALS AND METHODS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Growth of N. crassa and E. coli strains, plasmid constructs, and N. crassa electroporation:
All media were supplemented with 10 µg/ml pyridoxine-HCl.Media for his-3 strains contained 100 µg/ml histidine.Eight-day-old conidia isolated from Vogel's minimal medium (VM; VOGEL 1964 ) agar flasks were used to inoculate cultures forphysiological studies (DAVIS and DESERRES 1970 ). N. crassastrain genotypes are listed in Table 1. Escherichia coli strainDH5 ${alpha}$ was used to maintain all plasmids (HANAHAN 1983 ).

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Table 1. N. crassa strains

Two constitutively activating mutations, R178C and Q204L (JOHNSONet al. 1994 ), were made in gna-1 using site-directed mutagenesisessentially as previously described (KUNKEL et al. 1987 ). Theentire gna-1 gene region subcloned in pPNO5 (IVEY et al. 1996) is shown in Figure 1A; the template for mutagenesis (plasmidpPNO3) contained the 2.92-kb XhoI-ClaI fragment from this region.The presence of each mutation was verified by DNA sequencing(data not shown). To clone the Q204L mutation, a 2.67-kb EcoRI-XhoIfragment from pPNO2 (5' portion of gna-1; Figure 1A), a 0.89-kbXhoI-EcoRV fragment of the pPNO3 mutagenized replicative formDNA, and a 2.04-kb EcoRV-ClaI fragment from pPNO5 (see Figure1A) were inserted into pRAUW122 between the EcoRI and XbaI sites(XbaI made blunt with Klenow fragment). pRAUW122 is a vectorthat allows targeting to the his-3 locus of N. crassa (ARAMAYO1996 ; Figure 1A). To clone the R178C mutation, a 2.67-kb EcoRI-XhoIfragment from pPNO2 and a 2.92-kb XhoI-ClaI fragment from mutagenizedreplicative form pPNO3 DNA were inserted into pRAUW122 in themanner described for the Q204L mutation. A plasmid containingthe wild-type allele of gna-1 was constructed by insertion ofa 5.58-kb EcoRI-ClaI fragment (ClaI blunted using Klenow) frompPNO5 into pRAUW122 as described for the Q204L plasmid. Theplasmids containing the wild-type, Q204L, and R178C gna-1 allelesare designated as pQY17, pQY21, and pQY15, respectively.

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Figure 1. Construction of N. crassa strains with gna-1 alleles targeted to the his-3 locus. (A) Diagram of the his-3 region in the pRAUW122 plasmid, the gna-1 gene region in pPNO5, and targeting strategy. The top bar shows the genomic DNA insert of pRAUW122; the striped area is a portion of the his-3 gene. The bottom bar is the genomic DNA insert of pPNO5. The shaded area within the gna-1 gene region is the amino-acid coding sequence. The arrows below his-3 and gna-1 show the direction of translation. gna-1⁺, gna-1^R178C, and gna-1^Q204L alleles were inserted between the XbaI and EcoRI sites in the pRAUW122 polylinker as shown; the XbaI site of pRAUW122 and the ClaI site of gna-1 were made blunt with Klenow. The positions of various restriction enzyme sites are indicated. Enzyme abbreviations are as follows: H, HindIII; Xb, XbaI; EI, EcoRI; C, ClaI; EV, EcoRV; and Xh, XhoI. (B) Southern analysis of his-3 targeted homokaryotic strains. Genomic DNA was digested with HindIII and XbaI (lanes 1–3) or HindIII (lanes 4–10). The entire 8.8-kb insert from pRAUW122 depicted in A was used as a probe. Lanes 1 and 10 are the his-3 ${Delta}$ gna-1 recipient (R) strain 30-1; all other lanes are from his-3⁺ transformants. The relevant genotype of his-3⁺ strains is shown below the lane markings. Strains are lane 2, R-10-2; lane 3, R-5-7; lane 4, 17-7-7; lane 5, 17-3; lane 6, 15-9-2; lane 7, 15-38; lane 8, 21-5-1; and lane 9, 21-3-7. A 0.7-kb fragment was deleted from pRAUW122 during its construction (ARAMAYO 1996

); thus, the HindIII fragment containing the endogenous his-3 locus in strain 30-1 is larger than that resulting from vector integration (9.5 vs. 8.8 kb). Integration of gna-1 wild-type or activated alleles yields two 6.2-kb hybridizing fragments due to the presence of three HindIII sites in gna-1. After HindIII-XbaI digestion, the chromosomally encoded his-3 fragment is 9.5 kb, as there are no XbaI sites in this region. Integration of the his-3 vector without insert (for ${Delta}$ gna-1 negative controls) yields 5.2-kb and 3.6-kb fragments, due to cleavage of the XbaI site in the plasmid polylinker.

Electroporation of N. crassa (VANN 1995 ; IVEY et al. 1996) and gene-directed integration at the his-3 locus were performedas described (ARAMAYO 1996 ), with selection on sorbose-containingminimal medium (CASE et al. 1979 ). ${Delta}$ gna-1 strain 30-1 was therecipient (Table 1), and 2 µg pRAUW122, pQY17, pQY21,or PQY15 DNA was used for electroporation.

Southern and Western blot analysis:
Genomic DNA was isolated from transformants and subjected toSouthern analysis as described (SAMBROOK et al. 1989 ). The8.8-kb HindIII fragment of pRAUW122 was used as a probe. Toidentify strains with gna-1 wild-type or activated alleles atthe his-3 locus, genomic DNA was digested with HindIII. To identifystrains containing the his-3 targeting vector alone at the his-3locus, genomic DNA was digested with HindIII and XbaI.

Heterokaryotic transformants containing the correct-sized hybridizingfragments were purified to homokaryons by repeated plating onsorbose-containing plates. Southern analysis was used to verifythat in such homokaryons the endogenous his-3 fragment was replacedwith the appropriate vector sequences.

For plasma membrane isolation, conidia were inoculated intoliquid VM at a final concentration of 3.6 x 10⁶ conidia/ml.Cultures were incubated in the dark at 30° with shakingat 200 rpm for 16 hr. Mycelia were collected by filtration andcells were broken using a Bead-Beater (Biospec Products, Bartlesville,OK). The plasma membrane fraction was isolated and protein concentrationdetermined as described (TURNER and BORKOVICH 1993 ). Westernblot analysis of plasma membrane proteins was performed as described(BORKOVICH et al. 1989 ), using GNA-1, GNA-2, and GNB-1 antiserumat 1:1000, 1:300, and 1:5000 dilutions, respectively.

Phenotypic analysis:
Apical extension rates at 30° on normal and hyperosmoticmedium were determined as described (IVEY et al. 1996 ). Fordry weight accumulation measurements on solid media, VM platesoverlaid with cellophane were inoculated in the center withconidial suspensions. Plates were incubated at room temperaturein constant light for 3 days. The colonies were then scrapedfrom the plates onto filter paper and dried at 80° beforeweighing.

Sexual fertility assays were conducted on synthetic crossingmedium (SCM; WESTERGAARD and MITCHELL 1947 ) at room temperaturein constant light as described (IVEY et al. 1996 ). Strain 74Aconidia were used to fertilize protoperithecia on plates after10 days of growth.

cAMP and carotenoid pigment measurements:
To measure the in vivo cAMP levels of wild-type and mutant N.crassa cells, VM plates overlaid with cellophane were inoculatedwith conidial suspensions. Plates were incubated at room temperatureunder constant light for 3 days. Mycelial pads were scrapedfrom the plates, frozen in liquid nitrogen, and ground to afine powder. Powdered mycelia were suspended in 6% ice-coldtricarboxylic acid, and incubated on ice for at least 20 min.A 1-ml aliquot of each sample was centrifuged at 16,200 x gfor 25 min. The supernatant was chromatographed over a Dowex50W (H⁺ form) column and concentrated to purify cAMP as described(SALOMON et al. 1974 ). cAMP was quantitated using a competitivebinding protein assay as described (BROWN et al. 1971 ), withliquid scintillation counting in a Beckman LS 5801 counter (BeckmanInstruments, Fullerton, CA).

Mycelial pads, isolated as described above for the cAMP measurements,were lyophilized, weighed, ground to a fine powder, and extractedin 6 ml methanol for 20 min at 60°. After filtration, theresidue was reextracted with acetone for 20 min at 50° (PAIETTAand SARGENT 1981 ; LINDEN et al. 1997 ). The filtrates werecombined and the pigment content was estimated by optical densityon a DS-2000 Spectrophotometer (SLM Instruments, Urbana, IL).

Assays for sensitivity to heat and hydrogen peroxide:
Five-day-old conidia were inoculated into liquid VM medium ata concentration of 1 x 10⁶ cells/ml and germinated for 2 hrwith shaking at 200 rpm in the dark at 30°. For heat shockstudies, 1-ml samples were placed in glass tubes and held at30° (no induced thermotolerance) or given a 44° pretreatmentfor 30 min (to induce thermotolerance). Samples were then incubatedat 52° for 20 min (heat treatment). A control tube was alsoprepared that contained germlings incubated at 30° thatwere never subjected to a heat treatment (30° control).Aliquots were diluted and spread on sorbose plates, incubatedfor 2 to 3 days at 30°, and colonies counted. Percent survivalwas obtained by dividing the number of viable colonies afterheat treatment by the number on the 30° control plate, andmultiplying by 100.

For hydrogen peroxide sensitivity assays, 1-ml aliquots of 2-hrgermlings prepared as described above were brought up to 10mM hydrogen peroxide (final concentration) and incubated for2 hr at 30°. Samples were then diluted and plated on sorboseplates as described above. Percent survival was scored by dividingthe number of colonies obtained after peroxide treatment bythe number on a plate containing cells that were not exposedto hydrogen peroxide, and multiplying by 100.

RESULTS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Construction of isogenic strains and G protein analysis:
Previous studies have demonstrated that GNA-1 regulates severalprocesses during growth and development in N. crassa (IVEY etal. 1996 ); however, an active role for GNA-1 could not be assignedbased on the analysis of a ${Delta}$ gna-1 mutation alone. Therefore,to better characterize the function of GNA-1, we analyzed phenotypesin strains that contained null, wild-type, or activated (R178Cor Q204L) gna-1 alleles, but were otherwise isogenic. For constructionof these strains, we took advantage of an efficient gene targetingsystem for N. crassa that directs DNA sequences to the his-3locus (EBBOLE 1990 ; ARAMAYO 1996 ; Figure 1A). The constructsfor wild-type or activated gna-1 alleles all contained a 5.6-kbfragment of gna-1 genomic DNA previously shown to support expressionof the gene from ectopic sites (IVEY et al. 1996 ). Primaryheterokaryotic transformants and purified homokaryotic strainswere identified using Southern analysis (Figure 1B).

In mammalian cells, changes in expression of wild-type, inactivated,or activated G ${alpha}$ proteins can influence the expression of Gßproteins (HERMOUET et al. 1993 ). Altered expression of Gßor G ${alpha}$ proteins due to mutation of gna-1 could influence the phenotypesobserved in the N. crassa isogenic strains. Therefore, we determinedwhether activation of GNA-1 affected the expression of otherknown N. crassa G proteins. Levels of GNA-1, GNA-1^R178C, GNA-1^Q204L,GNA-2, and the only known N. crassa Gß protein, GNB-1(Q. YANG and K. BORKOVICH, unpublished results), were measuredin the isogenic strains using Western analysis (Figure 2). GNA-1and GNA-1^Q204L are expressed to the same level in the respectivestrains, but the GNA-1^R178C protein level is reduced ~50% (Figure2). The mobility of the GNA-1^R178C protein is also slightlyincreased relative to wild-type GNA-1. Expression of GNA-2 andGNB-1 was similar in wild-type, ${Delta}$ gna-1, gna-1^R178C, and gna-1^Q204Lstrains (Figure 2), indicating that mutationally activated gna-1alleles do not influence steady-state levels of other knownG protein subunits in N. crassa.

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Figure 2. Levels of GNA-1, GNA-2, and GNB-1 proteins. Samples containing 30 µg plasma membrane proteins were subjected to Western analysis as described in MATERIALS AND METHODS. Strains are 17-7-7 (gna-1⁺), 21-5-1 (gna-1^Q204L), 15-9-2 (gna-1^R178C), and R-10-2 ( ${Delta}$ gna-1). The migration positions of GNA-1, GNA-2, and GNB-1 are shown on the left side of the figure. GNA-1, GNA-2, and GNB-1 antibodies were used at dilutions of 1:1000, 1:300, and 1:5000, respectively.

Strains containing GTPase-deficient gna-1 alleles produce abundant, long aerial hyphae:
The colony morphology of ${Delta}$ gna-1, gna-1⁺, gna-1^R178C, and gna-1^Q204Lstrains was compared after growth on solid medium in light (Figure3A). Under these conditions, mycelia from N. crassa wild-typestrains produce aerial hyphae with conidiophores at their tips.These structures then give rise to asexual spores termed conidia(SPRINGER 1993 ; Figure 3A). As noted previously, ${Delta}$ gna-1 strainshave a reduced apical extension rate, producing smaller coloniesthan wild type (Figure 3A; IVEY et al. 1996 ). Furthermore,the ${Delta}$ gna-1 mutants produce fewer aerial hyphae per cross-sectionalarea than wild type (Figure 3A; data not shown). In contrast,the two strains with activating gna-1 mutations produce longer,more abundant aerial hyphae than wild type, with the greatestdensity seen in strains with the gna-1^Q204L allele (Figure 3A).In spite of the presence of more aerial hyphae, the activatedallele-containing strains produce the same amount (gna-1^R178C)or slightly fewer conidia than wild type (gna-1^Q204L; data notshown). Conversely, although the ${Delta}$ gna-1 strains possess feweraerial hyphae, they produce the same amount of conidia per cross-sectionalarea as wild-type controls (IVEY et al. 1995; data not shown).Thus, ${Delta}$ gna-1 mutants form more conidia per aerial hyphae thanwild type, while strains containing GTPase-deficient gna-1 allelesproduce fewer.

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Figure 3. Colony morphology and mass accumulation. (A) Colony morphology: Cellophane-overlaid VM plates were inoculated with conidia from the various strains and incubation at room temperature for 3 days in constant light. Strains are 17-7-7 (WT/wild type, gna-1⁺), 21-5-1 (gna-1^Q204L), 15-9-2 (gna-1^R178C), and R-10-2 ( ${Delta}$ gna-1). In this photograph aerial hyphae are the white fluffy material on the plate surface. (B) Relative mass on cellophane-overlaid VM plates. Strains are the same as in A. Values are expressed as the mean of the relative mass of wild type ± SEM from four independent experiments. Wild-type dry weight is 312.5 ± 28.3 mg.

We previously reported that wild-type strains accumulate moremass than ${Delta}$ gna-1 mutants, with the greatest effect seen aftergrowth in light (IVEY et al. 1996 ). On this basis, we predictedthat the synthesis of more aerial hyphae would result in greatermass for the gna-1^R178C and gna-1^Q204L strains. Therefore, wemeasured colony dry weights for the four strains after incubationin light (Figure 3B). As noted previously, ${Delta}$ gna-1 strains haveless mass than wild type (16.0% of wild type; Figure 3B). gna-1^R178Cand gna-1^Q204L strains accumulate greater mass than wild-typeor ${Delta}$ gna-1 mutant strains, with gna-1^Q204L weights the highest(160% of wild type; Figure 3B). Thus, the dry weight resultsroughly correlate with the appearance of aerial hyphae on plates.However, these experiments do not rule out the possibility thatdifferences in basal hyphae production among the various strainscould also contribute to the observed mass differences.

These results indicate that the aerial hyphae and dry weightphenotypes of ${Delta}$ gna-1, gna-1⁺, and gna-1^R178C and gna-1^Q204L strainsdiffer. Since Gß ${gamma}$ is predicted to be free in both ${Delta}$ gna-1and activated allele-containing strains, these results supporta Gß ${gamma}$ -independent role for GNA-1 during signaling. Furthermore,the increased aerial hyphae formation and dry weight accumulationobserved in strains with activating mutations suggest that GNA-1is a positive regulator of these processes. In contrast, activationof GNA-1 correlates with decreased conidia formation per aerialhyphae in N. crassa.

Activation of gna-1 does not greatly impact apical extension rate, osmotic sensitivity, or sexual fertility:
Previously we reported that ${Delta}$ gna-1 mutants are more sensitiveto hyperosmotic medium than wild type (IVEY et al. 1996 ). Therefore,we compared the osmotic sensitivity of ${Delta}$ gna-1, gna-1⁺, gna-1^R178C,and gna-1^Q204L strains after growth on solid medium containingno additions, or 1.5 M sorbitol, 0.75 M KCl, or 0.75 M NaCl(Table 2). In accordance with previous results (IVEY et al.1996 ), the ${Delta}$ gna-1 strain grew more slowly on both normal andhyperosmotic media than wild type (Table 2). In contrast, bothactivated alleles gave significant complementation of the ${Delta}$ gna-1defect, with the gna-1^R178C allele more effective than gna-1^Q204L(Table 2). These results are consistent with a Gß ${gamma}$ -independentrole for GNA-1 in regulation of apical extension rate on bothnormal and hyperosmotic media. Furthermore, the observationthat the osmotic tolerance of gna-1^R178C and gna-1^Q204L strainsis not greater than wild type implies that wild-type strainscannot increase their hyperosmotic tolerance through mutationalactivation of gna-1.

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Table 2. Relative growth rates on solid medium

In earlier studies, it was demonstrated that ${Delta}$ gna-1 strains aremale fertile, but female sterile (IVEY et al. 1996 ). To determineif GNA-1 plays a direct role in female fertility independentof Gß ${gamma}$ , we compared the ability of ${Delta}$ gna-1, wild-type, andactivated gna-1 allele-containing strains to serve as femaleparents during sexual crosses. As seen previously (IVEY et al.1996 ), ${Delta}$ gna-1 strains were female sterile, while wild-type strainswere fertile and produced perithecia containing viable ascosporesafter fertilization (Figure 4A and B; data not shown). gna-1^R178Cand gna-1^Q204L strains were female fertile, although these strainsproduced fewer and, on average, slightly larger perithecia thanwild type (Figure 4C and Figure D). Because the phenotypesof ${Delta}$ gna-1, wild-type, and activated-allele-containing strainsdiffer, GNA-1 plays an active role in regulating female fertilityin N. crassa. There was no effect on male fertility due to mutationof gna-1; all four strains could serve as male parents (datanot shown).

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Figure 4. Female fertility. SCM plates were inoculated with various strains, cultured to allow protoperithecial formation, and then fertilized using strain 74A conidia. Plates were photographed 7 days postfertilization. Strains are ${Delta}$ gna-1 R-10-2 (A); gna-1⁺ 17-7-7 (B); gna-1^R178C 15-9-2 (C); and gna-1^Q204L 21-3-7 (D). Examples of normal protoperithecia (small dark structures) and perithecia (larger, dark-colored spheres) can be seen in B for wild-type strain 17-7-7.

gna-1^R178C and gna-1^Q204L strains have lower carotenoid, but higher cAMP levels than wild-type strains:
In N. crassa, carotenoid synthesis is induced by blue lightin mycelia, whereas synthesis in conidia is constitutive (RAUand MITZKA-SCHNABEL 1985 ; BRAMLEY and MACKENZIE 1988 ). Previousstudies have demonstrated a negative correlation between cAMPlevels and carotenoid accumulation (KRITSKY et al. 1982 ). Inaddition, ${Delta}$ gna-1 strains have lower cAMP levels and are morepigmented than wild type (IVEY et al. 1996 ; D. IVEY and K.BORKOVICH, unpublished results). In this study, we observedthat carotenoid pigment production was visibly reduced in gna-1^R178Cand gna-1^Q204L colonies in comparison to wild type (Figure 3A).The lighter appearance of the gna-1^R178C and gna-1^Q204L strainsresults not only from reduced pigmentation in aerial and basalhyphae, but also from the production of fewer, less-pigmentedconidia (data not shown). Therefore, we extracted and quantitatedcarotenoids from ${Delta}$ gna-1, gna-1⁺, and gna-1^R178C and gna-1^Q204Lstrains grown in constant light. The spectrum of the extractedmaterial is indicative of carotenoids, with peaks at ~470 and495 nm (PAIETTA and SARGENT 1981 ; ARMSTRONG and HEARST 1996; Figure 5A). The ${Delta}$ gna-1 strain has the highest carotenoid content,whereas the two strains containing activated gna-1 alleles havelower carotenoid levels than wild type (Figure 5A).

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Figure 5. Carotenoid spectra and relationship between carotenoid and cAMP levels. (A) Absorbance spectra of carotenoid pigments: The visible absorption spectra of the carotenoid extracts were recorded and normalized to the dry weight of the original mycelial pad. The spectra peak at 470 and 495 nm. Strains are ${Delta}$ gna-1 R-10-2, gna-1⁺ 17-7-7, gna-1^R178C 15-9-2, and gna-1^Q204L 21-5-1. (B) Inverse correlation between cAMP and carotenoid pigment level: Strains are the same as in A. Values for cAMP and carotenoids were converted to percentage wild type before plotting. The cAMP value for wild type is 4.88 ± 0.55 pmoles/mg protein. Carotenoid levels are taken from Figure 5A, using the value of 470 nm for each strain. The carotenoid level of wild type is 7.48 absorbance units/g dry weight.

We have shown that deletion of gna-1 leads to lower adenylylcyclase activity and intracellular cAMP levels in cells grownon solid medium (D. IVEY, Q. YANG and K. BORKOVICH, unpublishedresults). To ascertain whether activation of gna-1 would leadto higher cAMP levels, we measured steady-state cAMP levelsin ${Delta}$ gna-1, gna-1⁺, and gna-1^R178C and gna-1^Q204L strains. Similarto previous results, the ${Delta}$ gna-1 strain has reduced levels ofcAMP (67.8% of wild type; see also Figure 5B). There is anincrease in cAMP levels in strains containing GTPase-deficientgna-1 alleles; gna-1^R178C strains have 123% and gna-1^Q204L strainshave 126% wild-type levels of cAMP (see also Figure 5B). Thus,there is a positive correlation among cAMP levels, aerial hyphaeformation, and GNA-1 activation state in N. crassa. In addition,the combined results from the carotenoid and cAMP assays demonstratean inverse relationship between cAMP and carotenoid levels inthe four strains (Figure 5B). Consistent with previous observations,our results support the hypothesis that aerial hyphae developmentis positively regulated by cAMP, but that lower cAMP levelspromote production of conidia and carotenoid accumulation (KRITSKYet al. 1982 ; MURAYAMA et al. 1995 ).

Strains containing GTPase-deficient gna-1 alleles exhibit increased sensitivity to heat and hydrogen peroxide-induced oxidative stress:
Carotenoids provide resistance to oxidative stress through quenchingof free radicals (KRINSKY 1992 ). In various fungal species,carotenoids are correlated with protection against oxidativestress (MOORE et al. 1989 ; SCHROEDER and JOHNSON 1995 ). Italso has been shown that exposure to oxidants can regulate synthesisof carotenoid pigments (SCHROEDER and JOHNSON 1995 ). As mentionedpreviously, resistance to oxidative stress is often linked toheat tolerance. Therefore, we measured the sensitivity of thefour strains to heat and to oxidative stress induced by hydrogenperoxide and paraquat.

Exposure of N. crassa cells to temperatures of 50° or aboveresults in significant lethality (KAPOOR 1983 ; PLESOFSKY-VIGand BRAMBL 1985 ; data not shown), while incubation at temperaturesbetween 40° and 47° leads to heat shock protein synthesisand significant retention of viability (KAPOOR 1983 ; PLESOFSKY-VIGand BRAMBL 1985 ). It has been demonstrated in N. crassa andother organisms that incubation of cells at sublethal heat shocktemperatures yields increased resistance to subsequent exposureto a lethal temperature; this phenomenon is termed induced thermotolerance(PLESOFSKY-VIG and BRAMBL 1985 ; LINDQUIST and CRAIG 1988 ).Induced thermotolerance is due at least in part to synthesisof heat shock proteins, which protect the cell from the normallylethal temperature (reviewed by MAGER and DE KRUIJFF 1995 ).

To assess thermotolerance in the N. crassa strains, we quantitatedsurvival after exposure to a 52° lethal heat treatment withand without prior exposure to the nonlethal heat shock temperatureof 44°. There was an inverse correlation between the extentof both uninduced and induced thermotolerance and the predictedGTP occupancy of the GNA-1 protein expressed in the four isogenicstrains (Figure 6A). ${Delta}$ gna-1 strains exhibited the greatest survivalafter heat treatment (10- to 35-fold more resistant than wildtype), while strains with GTPase-deficient alleles had the lowestsurvival (six times more sensitive than wild type). Thus, theactivation state of GNA-1 in N. crassa negatively influencessensitivity to heat.

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Figure 6. Sensitivity to heat and hydrogen peroxide. (A) Measurement of induced and uninduced thermotolerance: For uninduced thermotolerance, 2-hr germlings were incubated at 52° for 20 min, while induced thermotolerance was assessed by introducing a 30-min exposure to 44° before the 52° heat treatment. See MATERIALS AND METHODS for details. Strains are ${Delta}$ gna-1 R-10-2, gna-1⁺ 17-7-7, gna-1^R178C 15-9-2, and gna-1^Q204L 21-5-1. (B) Sensitivity to hydrogen peroxide: Two-hour germlings were incubated in 10 mM hydrogen peroxide at 30° for 2 hr. See MATERIALS AND METHODS for details. Strains are the same as in A.

We next measured viability in the presence of hydrogen peroxideto evaluate the oxidative stress response and found an inverserelationship between sensitivity to this oxidant and activationof GNA-1 (Figure 6B). ${Delta}$ gna-1 mutants are most resistant to 10mM hydrogen peroxide, with no killing observed under these conditions(104% viability). Wild-type strains exhibit 81.1% viability,while strains containing activating gna-1 alleles have 18.2–26.0%viability. In contrast to the above results, all four strainsexhibited essentially the same sensitivity to paraquat, a superoxide-generatingagent (data not shown). These findings suggest that GNA-1 negativelyregulates the activity or expression of enzymes important inthe defense against hydrogen peroxide but not superoxide.

DISCUSSION

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Previous work from our laboratory demonstrated that loss ofgna-1 leads to several phenotypes during the life cycle of N.crassa (IVEY et al. 1996 ). However, ${Delta}$ gna-1 strains are predictedto have increased free Gß ${gamma}$ levels, which can regulate downstreameffectors (SIMON et al. 1991 ). Hence, we could not concludethat the phenotypes of ${Delta}$ gna-1 strains directly resulted fromloss of effector regulation by GNA-1. In the present study,we explored the relationship between GNA-1 and Gß ${gamma}$ in signaltransduction by constructing a set of isogenic strains containingnull, wild-type, or activated gna-1 alleles. Because Gß ${gamma}$ would be free to signal in strains with either null or mutationallyactivated gna-1 alleles, a comparison of strain phenotypes wouldindicate whether GNA-1 possesses a Gß ${gamma}$ -independent rolein signaling. Our results demonstrate that ${Delta}$ gna-1, wild-type,and gna-1^R178C or gna-1^Q204L strains often have differing phenotypes,implying that GNA-1 has some functions independent of Gß ${gamma}$ in N. crassa. For example, apical extension rates on normaland hyperosmotic solid medium are similar for wild-type andactivated gna-1 allele-containing strains, while ${Delta}$ gna-1 strainshave substantially lower rates. Likewise, strains with wild-type,gna-1^R178C, or gna-1^Q204L genes have similar phenotypes duringthe sexual cycle, while ${Delta}$ gna-1 strains differ.

We also have identified several processes in which a more pronouncedphenotype is observed depending on the activated state of GNA-1:aerial hyphae formation, conidia production, dry weight accumulationon solid medium, carotenogenesis, sensitivity to heat shock,and resistance to hydrogen peroxide-induced oxidative stress.For example, ${Delta}$ gna-1 mutants elaborate fewer aerial hyphae, butare more resistant to heat and hydrogen peroxide treatment thanwild-type strains. In contrast, strains with mutationally activatedgna-1 alleles are superior to wild type in the first trait,but are more sensitive to heat and hydrogen peroxide. Theseresults suggest that the role of GNA-1 is dominant to Gß ${gamma}$ in these processes, with a greater concentration of GTP-boundGNA-1 leading to a stronger phenotype.

Our results demonstrate that GNA-1 has a profound effect onthe survival of N. crassa during exposure to lethal temperatures.One possible model to explain this observation is that GNA-1is a negative regulator of a heat-shock protein necessary forthermotolerance. At present, there is evidence for differentialexpression of various heat shock proteins during developmentalstages in N. crassa, including aerial hyphae development (FRACELLAet al. 1997 ; HAFKER et al. 1998 ). Thus, it is plausible thatthe regulatory roles of GNA-1 during aerial hyphae developmentand the heat stress response are related.

Oxidative metabolism is essential for the viability of obligateaerobes such as N. crassa. However, this metabolic state producessuperoxide, peroxide, and hydroxyl radicals, which are deleteriousto nucleic acids, proteins, and lipids (reviewed by MAGER andDE KRUIJFF 1995 ). Superoxide dismutases, catalases, and carotenoidpigments are key players in conferring resistance to these oxidantsin microorganisms (MOORE et al. 1989 ; MAGER and DE KRUIJFF1995 ). In N. crassa, a CuZn superoxide dismutase gene, dos-1,has been cloned, and properties of a null mutant have been characterized(CHARY et al. 1994 ). sod-1 null mutants are more sensitiveto paraquat than wild-type strains, but have normal viabilityafter a lethal heat treatment. Three forms of catalase havebeen identified in N. crassa, with differential regulation bydevelopmental stage, incubation at lethal temperatures, or paraquatexposure (CHARY and NATVIG 1989 ). Conidia from N. crassa albinostrains (lacking carotenoids) are more sensitive to singletoxygen (SHIMIZU et al. 1979 ). Our results suggest that GNA-1may regulate catalase and carotenoid biosynthetic enzyme activityor expression in N. crassa, while superoxide dismutase regulationis GNA-1 independent.

Increased production of reactive oxygen species is associatedwith all steps of conidiation in N. crassa: hyphal adhesion,aerial hyphae differentiation, and conidia formation (HANSBERGet al. 1993 ). It has been suggested that organisms that areunable to reduce reactive oxygen species use mechanisms to avoidoxygen that result in differentiation; in the absence of thesemechanisms they will die (HANSBERG and AGUIRRE 1990 ). Thus,the involvement of GNA-1 in aerial hyphae development and resistanceto hydrogen peroxide-induced oxidative stress may be linked;the oxidative stress response pathway is inhibited in strainswith GTPase-deficient gna-1 mutations, causing elevated sensitivityto hydrogen peroxide and hyperactivation of aerial hyphae formation.In this regard, it is of interest that Aspergillus nidulansstrains containing a GTPase-deficient allele of the gna-1 homologuefadA (fadA^G42R) do not produce aerial hyphae or conidia; insteadthey exhibit colony lysis (YU et al. 1996 ).

We have shown that deletion of gna-1 negatively influences adenylylcyclase activity and cAMP levels in N. crassa (D. IVEY, Q. YANGand K. BORKOVICH, unpublished results). In this study, we againdemonstrate that the ${Delta}$ gna-1 strain has lower cAMP levels thanwild type. We also show that the activated gna-1 allele-containingstrains have elevated levels of cAMP. It should be noted thatsteady-state, and not ligand-stimulated levels of cAMP, weremeasured in these experiments; the modest changes observed betweenthe various strains may reflect compensatory mechanisms thatmaintain cAMP levels at relatively constant levels (reviewedby BELTMAN et al. 1993 ; BURNS et al. 1996 ). Thus, the magnitudeof fluctuations in cAMP level induced by environmental signalsmay be much greater than the steady-state values suggest. Inaddition, the proposed involvement of GNA-1 in regulation ofcellular processes may involve both cAMP-dependent and -independentfunctions. For example, GNA-1 might regulate MAP kinase pathway(s)that respond to external stresses. In mammals, stress-activatedMAP kinase cascades have been identified (reviewed by PAULet al. 1997 ), and the osmostress response in S. cerevisiaeis mediated by the Hog1 MAP kinase pathway (BREWSTER et al.1993 ).

The formation of a multicellular organism and subsequent differentiationof specialized structures involves many genes and their products.The cellular machinery required to withstand environmental stressessuch as heat and oxidants is also regulated by numerous geneticloci. Our results are consistent with GNA-1 as a key mediatorof these interrelated processes in N. crassa. Future effortswill be directed toward elucidating the signal transductionpathways regulated by GNA-1 in performing these essential functions.

ACKNOWLEDGMENTS

We thank D. Ebbole and R. Aramayo for plasmids; J. Spudich andX.-C. Yu for preparation of figures; J. Spudich and E. Spudichfor use of equipment; and X.-N. Zhang and J. Sasaki for technicalassistance. We acknowledge J. Bieszke, D. Ivey, A. Kays, E.Spudich, and G. Turner for their critical comments on the manuscript.This work was supported by National Institutes of Health grantGM-48626 (to K.A.B.) and by an American Cancer Society JuniorFaculty Research Award JFRA-495 (to K.A.B.).

Manuscript received July 9, 1998; Accepted for publication September 29, 1998.

LITERATURE CITED

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

ARAMAYO, R., 1996 Gene replacements at the his-3 locus of Neurospora crassa.. Fungal Genet. Newsl. 43:9-13.

ARMSTRONG, G. A. and J. E. HEARST, 1996 Genetics and molecular biology of carotenoid pigment biosynthesis. FASEB J. 10:228-237[Abstract].

BELTMAN, J., W. K. SONNENBURG, and J. A. BEAVO, 1993 The role of protein phosphorylation in the regulation of cyclic nucleotide phosphodiesterases. Mol. Cell. Biochem. 127(128):239-253.

BIRNBAUMER, L., 1992 Receptor-to-effector signaling through G proteins: roles for ß ${gamma}$ dimers as well as ${alpha}$ subunits. Cell 71:1069-1072[Medline].

BORKOVICH, K. A., 1996 Signal transduction pathways and heterotrimeric G proteins, pp. 211–233 in The Mycota III: Biochemistry and Molecular Biology, edited by R. BRAMBL and G. A. MARZLUF. Springer-Verlag, Berlin/Heidelberg.

BORKOVICH, K. A., F. W. FARRELLY, D. B. FINKELSTEIN, J. TAULIEN, and S. LINDQUIST, 1989 HSP82 is an essential protein that is required in higher concentrations for growth of cells at higher temperatures. Mol. Cell. Biol. 9:3919-3930[Abstract/Free Full Text].

BRAMLEY, P. M. and A. MACKENZIE, 1988 Regulation of carotenoid biosynthesis. Curr. Top. Cell. Regul. 29:291-343[Medline].

BREWSTER, J. L., T. DE VALOIR, N. D. DWYER, E. WINTER, and M. C. GUSTIN, 1993 An osmosensing signal transduction pathway in yeast. Science 259:1760-1763[Abstract/Free Full Text].

BROWN, B. L., J. D. M. ALBANO, R. P. EKINS, and A. M. SGHERZI, 1971 A simple and sensitive saturation assay method for the measurement of adenosine 3':5'-cyclic monophosphate. Biochem. J. 121:561-562[Medline].

BRUNO, K. S., R. ARAMAYO, P. F. MINKE, R. L. METZENBERG, and M. PLAMANN, 1996 Loss of growth polarity and mislocalization of septa in a Neurospora mutant altered in the regulatory subunit of cAMP-dependent protein kinase. EMBO J. 15:5772-5782[Medline].

BURNS, F., A. Z. ZHAO, and J. A. BEAVO, 1996 Cyclic nucleotide phosphodiesterases: gene complexity, regulation by phosphorylation, and physiological implications. Adv. Pharmacol. 36:29-48.

CASE, M. E., M. SCHWEIZER, S. R. KUSHNER, and N. H. GILES, 1979 Efficient transformation of Neurospora crassa by utilizing hybrid plasmid DNA. Proc. Natl. Acad. Sci. USA 76:5259-5263[Abstract/Free Full Text].

CHARY, P. and D. O. NATVIG, 1989 Evidence for three differentially regulated catalase genes in Neurospora crassa: effects of oxidative stress, heat shock, and development. J. Bacteriol. 171:2646-2652[Abstract/Free Full Text].

CHARY, P., D. DILLON, A. L. SCHROEDER, and D. O. NATVIG, 1994 Superoxide dismutase (sod-1) null mutants of Neurospora crassa: oxidative stress sensitivity, spontaneous mutation rate and response to mutagens. Genetics 137:723-730[Abstract].

COLEMAN, D. E., A. M. BERGHUIS, E. LEE, M. E. LINDER, and A. G. GILMAN et al., 1994 Structures of active conformations of G_i ${alpha}$ ₁ and the mechanism of GTP hydrolysis. Science 265:1405-1412[Abstract/Free Full Text].

CRUZ, A. K., and H. F. TERENZI, J. A. JORGE, H. F. TERENZI, 1988 Cyclic AMP-dependent, constitutive thermotolerance in the adenylate cyclase-deficient cr-1 (crisp) mutant of Neurospora crassa.. Curr. Genet. 13:451-454[Medline].

DAVIS, R. H. and F. J. DESERRES, 1970 Genetic and microbiological research techniques for Neurospora crassa.. Methods Enzymol. 71A:79-143.

EBBOLE, D., 1990 Vectors for construction of translational fusions to ß-galactosidase. Fungal Genet. Newsl. 37:15-16.

FRACELLA, F., C. SCHOLLE, A. KALLIES, T. HAFKER, and T. SCHRODER et al., 1997 Differential HSC70 expression during asexual development of Neurospora crassa.. Microbiology 143:3615-3624[Medline].

FREISSMUTH, M. and A. G. GILMAN, 1989 Mutation of Gs alpha designed to alter the reactivity of the protein with bacterial toxins, substitutions at ARG187 result in loss of GTPase activity. J. Biol. Chem. 264:21907-21914[Abstract/Free Full Text].

GRAZIANO, M. P. and A. G. GILMAN, 1989 Synthesis in Escherichia coli of GTPase-deficient mutants of Gs alpha. J. Biol. Chem. 264:15475-15482[Abstract/Free Full Text].

GUPTA, S. K., C. GALLEGO, J. M. LOWNDES, C. M. PLEIMAN, and C. SABLE et al., 1992 Analysis of the fibroblast transformation potential of GTPase-deficient gip2 oncogenes. Mol. Cell. Biol. 12:190-197[Abstract/Free Full Text].

HAFKER, T., D. TECHEL, G. STEIER, and L. RENSING, 1998 Differential expression of glucose-regulated (grp78) and heat-shock-inducible (hsp70) genes during asexual development of Neurospora crassa.. Microbiology 144:37-43[Medline].

HANAHAN, D., 1983 Studies on transformation of Escherichia coli with plasmids. J. Mol. Biol. 166:557[Medline].

HANSBERG, W. and J. AGUIRRE, 1990 Hyperoxidant states cause microbial cell differentiation by cell isolation from dioxygen. J. Theor. Biol. 142:201-221[Medline].

HANSBERG, W., H. DE GROOT, and H. SIES, 1993 Reactive oxygen species associated with cell differentiation in Neurospora crassa.. Free Rad. Biol. Med. 14:287-293[Medline].

HARDING, R. W., 1973 Inhibition of conidiation and photoinduced carotenoid biosynthesis by cyclic AMP. Neurospora Newsl. 20:20-21.

HERMOUET, S., T. MURAKAMI, and A. M. SPIEGEL, 1993 Stable changes in expression or activation of G protein alpha i or alpha q subunits affect the expression of both beta 1 and beta 2 subunits. FEBS Lett. 327:183-188[Medline].

HUDSON, T. H., J. F. ROEBER, and G. L. JOHNSON, 1981 Conformational changes of adenylate cyclase regulatory proteins mediated by guanine nucleotides. J. Biol. Chem. 256:1459-1465[Free Full Text].

IVEY, F. D., P. N. HODGE, G. E. TURNER, and K. A. BORKOVICH, 1996 The G ${alpha}$ _i homologue gna-1 controls multiple differentiation pathways in Neurospora crassa.. Mol. Biol. Cell 7:1283-1297[Abstract].

JOHNSON, G. L., A. M. GARDNER, C. LANGE-CARTER, and N. QIAN, 1994 How does the G protein, G_i2, transduce mitogenic signals? J. Cell. Biochem. 54:415-422[Medline].

KAPOOR, M., 1983 A study of the heat-shock response in Neurospora crassa.. Int. J. Biochem. 15:639-649[Medline].

KRINSKY, N. I., 1992 Mechanism of action of biological antioxidants. Proc. Soc. Exp. Biol. Med. 200:248-254[Abstract].

KRITSKY, M. S., T. A. SOKOLOVSKY, T. A. BELOZERSKAYA, and E. K. CHERNYSHEVA, 1982 Relationship between cyclic AMP level and accumulation of carotenoid pigments in Neurospora crassa.. Arch. Microbiol. 133:206-208.

KUNKEL, T. A., J. D. ROBERTS, and R. A. ZAKOUR, 1987 Rapid and efficient site-specific mutagenesis without phenotypic selection. Methods Enzymol. 154:367-382[Medline].

KURJAN, J., 1992 Pheromone response in yeast. Annu. Rev. Biochem. 61:1097-1129[Medline].

LINDEN, H., M. RODRIGUEZ-FRANCO, and G. MACINO, 1997 Mutants of Neurospora crassa defective in regulation of blue light perception. Mol. Gen. Genet. 254:111-118[Medline].

LINDQUIST, S. and E. A. CRAIG, 1988 The heat-shock proteins. Annu. Rev. Genet. 22:631-677[Medline].

MAGER, W. H. and A. J. J. DE KRUIJFF, 1995 Stress-induced transcriptional activation. Microbiol. Rev. 59:506-531[Abstract/Free Full Text].

MARCHLER, G., C. SCHULLER, G. ADAM, and H. RUIS, 1993 A Saccharomyces cerevisiae UAS element controlled by protein kinase A activates transcription in response to a variety of stress conditions. EMBO J. 12:1997-2003[Medline].

MOORE, M. M., M. W. BREEDVELD, and A. P. AUTOR, 1989 The role of carotenoids in preventing oxidative damage in the pigmented yeast, Rhodotorula mucilaginosa.. Arch. Biochem. Biophys. 270:419-431[Medline].

MURAYAMA, T., Y. FUJISAWA, and Y. OKANO, 1995 A suppressor mutation which suppresses adenylyl cyclase mutations in Neurospora crassa.. Exp. Mycol. 19:320-323[Medline].

PAIETTA, J. and M. L. SARGENT, 1981 Photoreception in Neurospora crassa: correlation of reduced light sensitivity with flavin deficiency. Proc. Natl. Acad. Sci. USA 78:5573-5577[Abstract/Free Full Text].

PAUL, A., S. WILSON, C. M. BELHAM, C. J. M. ROBINSON, and P. H. SCOTT et al., 1997 Stress-activated protein kinases: activation, regulation and function. Cell. Signalling. 9:403-410[Medline].

PLESOFSKY-VIG, N. and R. BRAMBL, 1985 Heat shock response of Neurospora crassa: protein synthesis and induced thermotolerance. J. Bacteriol. 162:1083-1091[Abstract/Free Full Text].

RAU, W. and U. MITZKA-SCHNABEL, 1985 Carotenoid synthesis in Neurospora crassa.. Methods Enzymol. 110:253-267[Medline].

SALOMON, Y., C. LONDOS, and M. RODBELL, 1974 A highly sensitive adenylate cyclase assay. Anal. Biochem. 58:541-548[Medline].

SAMBROOK, J., E. F. FRITSCH and T. MANIATIS, 1989 Molecular Cloning: A Laboratory Manual. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, NY.

SCHROEDER, W. A. and E. A. JOHNSON, 1995 Singlet oxygen and peroxyl radicals regulate carotenoid biosynthesis in Phaffia rhodozyma.. J. Biol. Chem. 270:18374-18379[Abstract/Free Full Text].

SHIMIZU, M., T. EGASHIRA, and U. TAKAHAMA, 1979 Inactivation of Neurospora crassa conidia by singlet molecular oxygen generated by a photosensitized reaction. J. Bacteriol. 138:293-296[Abstract/Free Full Text].

SHIN, D. Y., K. MATSUMOTO, H. IIDA, I. UNO, and T. ISHIKAWA, 1987 Heat shock response of Saccharomyces cerevisiae mutants altered in cyclic AMP-dependent protein phosphorylation. Mol. Cell. Biol. 7:244-250[Abstract/Free Full Text].

SIMON, M. I., M. P. STRATHMANN, and N. GAUTAM, 1991 Diversity of G proteins in signal transduction. Science 252:802-808[Abstract/Free Full Text].

SPRINGER, M. L., 1993 Genetic control of fungal differentiation: the three sporulation pathways in Neurospora crassa.. Bioessays 15:365-374[Medline].

TERENZI, H. F., M. M. FLAWIA, and H. N. TORRES, 1974 A Neurospora crassa morphological mutant showing reduced adenylate cyclase activity. Biochem. Biophys. Res. Commun. 58:990-996[Medline].

TURNER, G. E. and K. A. BORKOVICH, 1993 Identification of a G protein ${alpha}$ subunit from Neurospora crassa that is a member of the G_i family. J. Biol. Chem. 268:14805-14811[Abstract/Free Full Text].

VANN, D. C., 1995 Electroporation-based transformation of freshly harvested conidia of Neurospora crassa.. Fungal Genet. Newsl. 42A:53.

VOGEL, H. J., 1964 Distribution of lysine pathways among fungi: evolutionary implications. Am. Nat. 98:435-446.

WESTERGAARD, M. and H. K. MITCHELL, 1947 Neurospora V. A synthetic medium favoring sexual reproduction. Am. J. Bot. 34:573-577.

YARDEN, O., M. PLAMANN, D. J. EBBOLE, and C. YANOFSKY, 1992 cot-1, a gene required for hyphal elongation in Neurospora crassa, encodes a protein kinase. EMBO J. 11:2159-2166[Medline].

YU, J. H., J. WIESER, and T. H. ADAMS, 1996 The Aspergillus FlbA RGS domain protein antagonizes G protein signaling to block proliferation and allow development. EMBO J. 15:5184-5190[Medline].

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