Identification of vib-1, a Locus Involved in Vegetative Incompatibility Mediated by het-c in Neurospora crassa

Identification of vib-1, a Locus Involved in Vegetative Incompatibility Mediated by het-c in Neurospora crassa

Qijun Xiang^a and N. Louise Glass^a
^a Department of Plant and Microbial Biology, University of California, Berkeley, California 94720-3102

Corresponding author: N. Louise Glass, University of California, Berkeley, CA 94720-3102., lglass{at}uclink.berkeley.edu (E-mail)

Communicating editor: M. SACHS

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

A non-self-recognition system called vegetative incompatibilityis ubiquitous in filamentous fungi and is genetically regulatedby het loci. Different fungal individuals are unable to formviable heterokaryons if they differ in allelic specificity ata het locus. To identify components of vegetative incompatibilitymediated by allelic differences at the het-c locus of Neurosporacrassa, we isolated mutants that suppressed phenotypic aspectsof het-c vegetative incompatibility. Three deletion mutantswere identified; the deletions overlapped each other in an ORFnamed vib-1 (vegetative incompatibility blocked). Mutationsin vib-1 fully relieved growth inhibition and repression ofconidiation conferred by het-c vegetative incompatibility andsignificantly reduced hyphal compartmentation and death rates.The vib-1 mutants displayed a profuse conidiation pattern, suggestingthat VIB-1 is a regulator of conidiation. VIB-1 shares a regionof similarity to PHOG, a possible phosphate nonrepressible acidphosphatase in Aspergillus nidulans. Native gel analysis ofwild-type strains and vib-1 mutants indicated that vib-1 isnot the structural gene for nonrepressible acid phosphatase,but rather may regulate nonrepressible acid phosphatase activity.

FILAMENTOUS fungi grow by hyphal tip extension and branching.Within the interior of a colony, hyphae undergo fusion to forma network that makes up the fungal individual (BULLER 1933 ; GLASS et al. 2000 ; HICKEY et al. 2002 ). Filamentous fungican also undergo hyphal fusion between isolates, resulting inthe formation of a heterokaryon, in which genetically differentnuclei coexist in a common cytoplasm. The viability of suchheterokaryons, however, is genetically controlled by a numberof loci, termed het (for heterokaryon) or vic (vegetative incompatibility; GLASS and KULDAU 1992 ; LESLIE 1993 ). In heterokaryotic cells,a genetic difference in allelic specificity at any het locusbetween two fungal strains causes a phenomenon called vegetativeincompatibility (GLASS et al. 2000 ; SAUPE 2000 ). In manyfungal species, a macroscopic barrage forms when two incompatibleindividuals meet (ESSER and BLAICH 1994 ), which is caused byabnormal or lethal hyphal fusions in the area of contact. Vegetativeincompatibility also can be triggered in forced heterokaryons,partial diploids, or transformants that contain het allelesof alternative specificity (MYLYK 1975 ; PERKINS 1975 ; SAUPEand GLASS 1997 ; WU and GLASS 2001 ). In pseudohomothallicfungal species, self-incompatible progeny can be obtained fromcrosses between two incompatible parents (SAUPE 2000 ; SAENZet al. 2001 ). Phenotypic aspects of vegetative incompatibilityinclude hyphal compartmentation and death (HCD), lack of conidiation(in species that produce conidia), and growth inhibition (GARNJOBSTand WILSON 1956 ; BOUCHERIE and BERNET 1978 ; JACOBSON etal. 1998 ; WU and GLASS 2001 ).

Vegetative incompatibility has been studied extensively in twoascomycete species, Neurospora crassa and Podospora anserina(for reviews, see GLASS et al. 2000 ; SAUPE 2000 ). A totalof 9 het loci in P. anserina and 11 het loci in N. crassa havebeen described. Genes at 4 het loci in N. crassa and 3 het lociin P. anserina have been cloned. The predicted protein productsof these het loci are diverse. N. crassa het-c and het-6 andP. anserina het-s and het-e are not essential for cellular processesother than vegetative incompatibility. They encode a plasmamembrane protein, a putative protein, a prion analog, a proteinwith a GTP-binding site, and a C-terminal WD repeat domain,respectively (TURCQ et al. 1990 ; SAUPE et al. 1995 , SAUPEet al. 1996 ; SMITH et al. 2000). The other three het loci encodeproteins involved in biological processes in addition to vegetativeincompatibility. The N. crassa mating-type genes, mat A-1 andmat a-1, regulate mating and vegetative incompatibility andencode putative transcriptional factors with predicted DNA-bindingdomains (GLASS et al. 1990 ; STABEN and YANOFSKY 1990 ). Theun-24 locus encodes a polypeptide with high identity to thelarge subunit of type I ribonucleotide reductase (SMITH et al.2000A , SMITH et al. 2000B ), which catalyzes the synthesisof deoxyribonucleotides that are required for DNA replicationand repair (JORDAN and REICHARD 1998 ). P. anserina het-c encodesa putative glycolipid transfer protein required for ascosporematuration (SAUPE et al. 1994 ).

Mutations that relieve vegetative incompatibility have alsobeen identified in these two species. Mutations at the tol locussuppress mating-type vegetative incompatibility in N. crassa(NEWMEYER 1970 ; VELLANI et al. 1994 ), and tol mutations donot affect vegetative incompatibility mediated by other hetloci (LESLIE and YAMASHIRO 1997 ). tol encodes a putative protein(SHIU and GLASS 1999 ) that shares three conserved amino acidregions with HET-6 in N. crassa and HET-E in P. anserina (SMITHet al. 2000). In P. anserina, mod (for modifier) mutants thatsuppress some phenotypic aspects of vegetative incompatibilityhave been described (SAUPE 2000 ). Mutations in mod-A relievegrowth inhibition caused by interactions between nonallelichet loci, but cannot fully relieve HCD (BELCOUR and BERNET 1969). Complete suppression of vegetative incompatibility in a mod-Amutant requires a second mutation at the mod-B locus. mod-Ahas been cloned and encodes a novel protein (BARREAU et al.1998 ). Mutations at another mod locus, mod-C, suppress nonallelicvegetative incompatibility between het-R and het-V, but notother nonallelic incompatibility interactions. mod mutants alsoshow morphological or developmental defects. Extragenic mutations(mod-D through mod-G) that suppress these morphological or developmentaldefects have been identified. Two of these genes, mod-D andmod-E-1, have been characterized at the molecular level. Theyencode an ${alpha}$ -subunit of trimeric G protein and HSP90, respectively(LOUBRADOU et al. 1997 , LOUBRADOU et al. 1999 ).

The het-c locus in N. crassa has been used as a model systemto understand molecular mechanisms of non-self-recognition (SAUPEet al. 1996 ; SAUPE and GLASS 1997 ; WU and GLASS 2001 ) andto assess selection mechanisms for polymorphisms at het loci(WU et al. 1998 ; MUIRHEAD et al. 2002 ). The het-c locus encodesthree allelic specificities, termed het-c^OR, het-c^PA, and het-c^GR(nomenclature is based on het-c allelic specificity of laboratorystrains). The polypeptides encoded by the three het-c allelicspecificities are similar except for a variable domain of $~$ 34–48amino acids. This polymorphic region is necessary and sufficientto confer het-c allelic specificity (SAUPE and GLASS 1997 ; WU and GLASS 2001 ). HET-C is a plasma membrane protein; non-self-recognitionis correlated with the formation of a HET-C heterocomplex composedof HET-C polypeptides of alternative specificity (S. SARKAR,G. IYER and N. L. GLASS, unpublished data).

In an effort to identify components of vegetative incompatibilityin addition to het-c, we identified a number of mutants thatsuppressed het-c vegetative incompatibility. Previously, wereported on the isolation of a mutant (ahc) identified froma strain that had "escaped" from het-c vegetative incompatibility(XIANG et al. 2002 ). "Escape" is a process whereby strainsthat contain het alleles of alternative specificity (and displayslow, aconidial growth) recover to wild-type-like growth (fastergrowth and conidiation). The escape process has been associatedwith deletions and point mutations in genes that relieve vegetativeincompatibility, such as within the het locus itself, or insuppressor loci (NEWMEYER 1970 ; DELANGE and GRIFFITHS 1975; SMITH et al. 1996 ; COUSTOU et al. 1999 ). The ahc mutantcarries a large deletion ( $~$ 26 kbp) covering a number of predictedopen reading frames (ORFs), including a locus, ham-2, whichis required for hyphal fusion (XIANG et al. 2002 ). The introductionof ham-2 into the ahc mutant complemented morphological defects,such as the lack of aerial hyphae formation and hyphal fusion,but did not complement het-c vegetative incompatibility, indicatingthat a different ORF in the deletion region of the ahc mutantwas required for this process. In this study, we isolated twoadditional mutants, vc1 and vc2 (for vegetative incompatibilityand conidiation), from other escape strains that suppressedhet-c-mediated vegetative incompatibility. The mutations invc1 and vc2 were also deletions in the same chromosomal regionas the ahc deletion; the three deletions overlapped in a regioncovering an ORF. Mutations in this ORF (named vib-1, for vegetativeincompatibility blocked) restored growth and conidiation inhet-c incompatible heterokaryons, but only partially suppressedHCD.

MATERIALS AND METHODS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

N. crassa strains and heterokaryon tests:
The strains used in this study are listed in Table 1. Strainswere cultured on Vogel's medium (VOGEL 1964 ) with supplementsas required. Strains were cultured at 25° in 30- or 50-cm-longrace tubes to measure growth rates. Crosses were performed onWestergaard's medium (WESTERGAARD and MITCHELL 1947 ). Moststrains constructed in this study carry auxotrophic markers.To improve the fertility of these strains, 5–10% of recommendedamounts of corresponding supplements for vegetative growth wasadded to the crossing medium or, alternatively, the helper strainFGSC 4564 (PERKINS 1984 ) was used to form heterokaryons, whichwere subsequently used as female strains in crosses. Heterokaryontests were performed by co-inoculating 1–2 µl eachfrom conidial suspensions ( $~$ 10⁵ conidia/µl) of two differentauxotrophic strains onto plates or race tubes containing Vogel'smedium (VOGEL 1964 ).

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Table 1. N. crassa strains

Nucleic acid isolation, Southern hybridization, PCR, and DNA sequence analysis:
Genomic DNA was isolated as described (LEE and TAYLOR 1990 ).Southern hybridization was performed as described (SAMBROOKet al. 1989 ). Primers used to amplify an internal fragment( $~$ 800 bp) of het-c from the escape transformants were 5'-GGAGACATGGCGATATCG-3'and 5'-CTCACCCAACACGGAGTG-3'. The het-c^OR and het-c^PA PCR productswere distinguishable by ApaI digestion. The het-c^OR PCR fragmenthas an ApaI site, while an ApaI site is absent in the het-c^PAPCR fragment. Primers used to amplify mutated regions from vib-1^ripmutants were 5'-AATCCGGTGCAGATGAATACTG-3' at position 54–75bp downstream of the start codon in the vib-1 ORF and 5'-ATCTGCTTCGCAGACGTGAACGT-3'at position 1249–1272 bp downstream of the start codonin the vib-1 ORF. DNA sequence determinations were performedusing the ABI automated DNA sequencing procedure at DNA SequencingFacility, Berkeley, California (http://idrive.berkeley.edu/dnaseq/web).

Gene cloning:
DNA sequences of cosmid H57:G1 (XIANG et al. 2002 ) were fromthe Munich Information Centre for Protein Sequences (MIPS; http://www.mips.biochem.mpg.de/proj/neurospora/).DNA fragments carrying the vib-1 ORF were subcloned from cosmidH57:G1 into plasmid pCB1004, which confers hygromycin resistance(CARROLL et al. 1994 ). Spheroplast isolation and transformationwere performed as described (SCHWEIZER et al. 1981 ).

Hyphal compartmentation and death assay:
Sterile pieces of cellophane (Fisher Scientific) were spreadonto the surface of solid medium. Heterokaryons were forcedby co-inoculating conidia of two strains ( $~$ 10⁵ conidia from eachstrain) onto the cellophane. At different time points afterinoculation, the cellophane containing hyphae was peeled offfrom the surface of the medium and stained with 1% Evan's Blue(GAFF and OKONG'O-OGOLA 1971 ; JACOBSON et al. 1998 ). Stainedhyphae were examined under bright field using a Zeiss AxioskopII microscope.

Native PAGE analysis of phosphatases:
All strains were cultured in liquid Vogel's medium (phosphaterich; VOGEL 1964 ) with corresponding supplements at 30°for 2 days. Cultures were subsequently transferred to eitherhigh-phosphate or low-phosphate conditions with constant shaking(100 rpm) at 30° overnight. For high-phosphate conditions,the liquid medium was replaced with fresh phosphate-rich Vogel'smedium (VOGEL 1964 ). For low-phosphate conditions, the hyphaewere washed thoroughly with distilled water and subsequentlytransferred to phosphate-depleted Vogel's medium, plus 0.05mM KH₂PO₄. Harvesting of mycelia, protein extraction, and 8%polyacrylamide gel electrophoresis were performed as described(HOCHBERG and SARGENT 1973 ). Phosphatase activity was examinedas described (DORN 1965 ) with minor modifications: the gelwas flooded with 0.6 M acetate buffer (pH 4.8) containing 0.05%sodium ${alpha}$ -naphthyl acid phosphate (Sigma, St. Louis) plus 0.5%fast garnet G. B. C salt (Aldrich Chemical, Milwaukee) for 1hr at room temperature. During staining, sodium ${alpha}$ -naphthyl acidphosphate is converted into ${alpha}$ -naphthol and phosphate by phosphatases. ${alpha}$ -Naphthol forms an insoluble dark-brown compound with fast garnetG. B. C salt, which is deposited where phosphatases are locatedin the gel. The reaction was terminated by washing the gel thoroughlywith distilled water.

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Identifying suppressors of het-c vegetative incompatibility:
Our strategy to identify additional components of vegetativeincompatibility was to isolate mutants that suppressed the phenotypicaspects of het-c vegetative incompatibility, namely growth inhibition,repression of conidiation, and HCD. Incompatible partial diploids,heterokaryons, or transformants that contain het alleles ofalternative specificity commonly escape from vegetative incompatibilityafter being maintained in culture for $~$ 2 weeks. The escape processis associated with a sudden increase in conidiation and growthrate of the cultures. Escape has been associated with mutationseither in one of the het alleles or at a locus required to mediatevegetative incompatibility (NEWMEYER 1970 ; DELANGE and GRIFFITHS1975 ; VELLANI et al. 1994 ; SMITH et al. 1996 ). In our study,the het-c^OR allele in plasmid pCB1004 (which confers hygromycinresistance; CARROLL et al. 1994 ) was transformed into C9-2(het-c^PA thr-2 a; Table 1). Approximately 90 hygromycin-resistantincompatible transformants were transferred to slants. Sixtyescape transformants were analyzed. Heterokaryon tests and PCRanalysis of these escape transformants showed that 24 isolatescontained only one het-c allele, either het-c^OR or het-c^PA.The other 36 escape transformants maintained both het-c^OR andhet-c^PA alleles (data not shown). The coexistence of both het-calleles in these escape transformants suggested that extragenicmutations had occurred that suppressed the phenotypic aspectsof het-c vegetative incompatibility.

To identify the genetic basis of the escape phenotype in transformantsretaining both het-c^OR and het-c^PA, 14 escape transformantswere crossed with RLM 57-30 (het-c^OR pyr-4 A; Table 1). Allof the escape transformants were fertile as males except forb-11-1, which showed greatly reduced fertility (XIANG et al.2002 ). We selected for pyr-4 progeny (and thus het-c^OR, towhich pyr-4 is closely linked). Heterokaryons were forced betweenpyr-4 a progeny from each cross and the parental escape transformant[genotype: het-c^PA (pCB1004::het-c^OR) thr-2 a]. If a suppressormutation was not linked to het-c, the ratio of pyr-4 progenyforming compatible vs. incompatible heterokaryons with the parentalescape transformant should be $~$ 1:1. In 11 crosses, all pyr-4progeny ( $~$ 20 progeny from each cross) were incompatible withtheir parental escape transformants. These mutants presumablycontained mutations linked to het-c on LGII (which was selectedagainst in this cross) that suppressed vegetative incompatibilityor vegetative incompatibility was suppressed by epigenetic mechanismsin the original escape transformants and was not inherited bythe progeny. The twelfth cross (b-11-1 x RLM 57-30) led to theidentification of the ahc mutant (XIANG et al. 2002 ). In theremaining two crosses (b-19-5 x RLM 57-30) and (c3-1 x RLM 57-30),half of the pyr-4 a progeny formed compatible heterokaryonswith their parental transformants, b-19-5 or c3-1, respectively.These results suggested that b-19-5 and c3-1 carried mutationsunlinked to het-c that suppressed het-c vegetative incompatibility.

Phenotypic characterization of the suppressors:
The pyr-4 progeny from the above crosses that formed compatibleheterokaryons with b-19-5 or c3-1 showed a similar phenotypeof profuse conidiation (Fig 1A; 9-39-10 is descended from b-19-5and 24-24-9 is descended from c3-1). Approximately one-halfof the thr-2 progeny (from both b-19-5 and c3-1 crosses withRLM 57-30) also showed a profuse conidiation phenotype, suggestingthat the mutation that resulted in the profuse conidiation phenotypein these progeny was unlinked to pyr-4 or thr-2 (left arm ofLGII, linked to het-c).

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Figure 1. Morphological phenotype of the ahc, vc, and vib-1 mutants as compared to a wild-type strain. (A) The phenotype of the 8-88 (ahc), 9-39-10 (vc1), 24-24-9 (vc2), and 80-32 (vib-1(1)) mutant strains as compared to wild type when grown on petri plates. Conidiation in a wild-type strain occurs around the perimeter of the plate, while the ahc, vc, and vib-1 mutants produce profuse conidia across the plates. (B) The growth rates of ahc, vc, and vib-1(1) mutants as compared to a wild-type strain.

To determine whether the profuse conidiation phenotype segregatedwith suppression of vegetative incompatibility, a thr-2 het-c^PAprogeny from b-19-5 x RLM 57-30 showing the profuse conidiationpattern was crossed with RLM 57-30; 74 progeny were analyzed.Thirty-five progeny from the cross showed the profuse conidiationpattern, while the rest of progeny were wild type in phenotype.Progeny carrying the thr-2 (and thus het-c^PA) or the pyr-4 (andthus het-c^OR) marker were recovered. The pyr-4 het-c^OR progenywith the profuse conidiation phenotype were forced in heterokaryonswith thr-2 het-c^PA progeny with the profuse conidiation phenotype(same mating-type pairing). The conidiation pattern of the resultingheterokaryons and their growth rates were indistinguishablefrom the mutants by themselves (Fig 2, A and B, heterokaryon(9-39-10 + 9-39-7); Fig 1A and Fig B). Analysis of crosseswith c3-1 yielded similar results. We named the mutants carryingthese mutations as vc1 (mutants derived from escape transformantb-19-5) and vc2 (for mutants derived from escape transformantc3-1).

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Figure 2. vib-1 mutants relieve repression of conidiation and growth inhibition associated with het-c vegetative incompatibility. (A) A compatible heterokaryon (9-1-5 + FGSC 4564) and a het-c incompatible heterokaryon (FGSC 4564 + C9-2). A heterokaryon between a het-c^OR; vib-1(1) (X80-32) and a het-c^PA; vib-1(1) (X80-49) strain shows profuse conidiation. Similarly, a vc1 heterokaryon [het-c^OR; vc1 (9-39-10) + het-c^PA; vc1 (9-39-7)] also shows profuse conidiation. (B) The vib-1 and vc1 mutations suppress growth rate inhibition mediated by allelic specificity differences at het-c and have growth rates similar to the mutants themselves (Fig 1B). The numbers below the columns indicate the heterokaryons with the same numbers shown in A. Standard error bars are shown. (C) The semirecessive nature of vc1 suppression of het-c vegetative incompatibility. The wild-type het-c incompatible heterokaryon is (I-1-51 + Xa-2). The heterokaryon developed conidia in a small section of the plate on the ninth day, which was possibly due to mutational processes resulting in escape. A compatible heterokaryon (I-1-51 + FGSC 4564) is also shown. The middle panel shows a heterokaryon between a het-c^OR; vc1 strain and a het-c^PA strain (9-39-10 + Xa-2). Conidiation was observed on the fourth day and spread across the plate by the ninth day.

In race tubes under normal laboratory conditions, the vc1 andvc2 mutants formed dense patches of conidia along the lengthof 50-cm race tubes that later filled in to form a continuousconidial mat. By contrast, a wild-type strain forms dense conidialpatches only at the two ends of the race tube; conidiation inthe middle of the race tube is suppressed by a high concentrationof CO₂ (SARGENT et al. 1972 ). The vc1 and vc2 mutants havea slightly slower growth rate, 4–5 cm/day as comparedto 6–7 cm/day for a wild-type strain (Fig 1B).

To determine whether the vc1 and vc2 mutations were recessiveor dominant, heterokaryons were forced between the vc1 and vc2mutants and wild-type strains with het-c alleles of the sameor alternative het-c allelic specificity. Heterokaryons betweena wild-type strain (FGSC 4564; Table 1) and the vc1 or vc2mutants (9-39-10 or 24-24-9) of identical het-c specificitydisplayed wild-type growth rates and a normal conidiation pattern,indicating that the morphological phenotype of the vc1 and vc2mutants was recessive (data not shown). Heterokaryons betweenhet-c^OR; vc1 or het-c^OR; vc2 mutants with a wild-type het-c^PAstrain (Xa-2; Table 1) displayed typical het-c vegetative incompatibilityduring the first 3 days. However, after 4 days an increase ingrowth rate was observed in the heterokaryons and conidiationbegan in the middle of the plate (Fig 2C). By contrast, an increasein growth rate and conidiation was not observed in wild-typehet-c incompatible heterokaryons. These results indicate thatthe suppression of het-c vegetative incompatibility by the vc1and vc2 mutations was not completely recessive.

Complementation between suppressor mutants:
The ahc, vc1, and vc2 mutants all show suppression of het-cvegetative incompatibility and have a similar phenotype, althoughthe ahc mutant has additional morphological defects. The ahcmutant is female sterile, shows ascus-dominant developmentaldefects, and is severely restricted in its capacity to undergohyphal fusion (XIANG et al. 2002 ). Heterokaryon tests wereperformed to determine if the three mutants can complement eachother's morphological defects. A heterokaryon between an ahcmutant (X39-12) and vc1 (9-39-10) or vc2 (24-24-9) mutants (usinga modified heterokaryon test; XIANG et al. 2002 ) of identicalhet-c specificity showed the morphology of a vc1 or vc2 mutant.Although the slow mycelial growth of the ahc mutant was complementedin a heterokaryon with the vc1 or vc2 mutant, the profuse conidiationpattern was not. A heterokaryon between vc1 mutant (X43-12)and vc2 mutant (24-24-9) displayed a similar growth rate andconidiation pattern of vc1 or vc2 mutants themselves. The aboveresults suggest that the mutations resulting in the conidiationdefect in ahc, vc1, and vc2 mutants were allelic. We previouslymapped the mutation in the ahc mutant to chromosome V betweenlys-2 and ilv-2 (XIANG et al. 2002 ).

All three suppressor mutants carry deletions that overlap in an ORF:
The ahc mutant carries a deletion covering at least eight predictedORFs, including ham-2, a locus involved in hyphal fusion (XIANGet al. 2002 ). Southern hybridization was performed to determinewhether vc1 and vc2 mutants also carried deletions in this region.Probes were generated from cosmid H57:G1, which was previouslyshown to span most of the deletion in the ahc mutant (XIANGet al. 2002 ). Fig 3 shows that the 6280-bp HindIII fragmentcarrying ham-2 was present in both vc1 and vc2 mutants. However,a 5278-bp HindIII fragment is completely absent from the vc1mutant. Most of this fragment is also absent from vc2. In theahc mutant, both HindIII fragments are missing.

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Figure 3. Southern blots showing the vib-1 region in the ahc, vc1, and vc2 deletion mutants. (A) Restriction enzyme sites in the region covering ham-2 and vib-1. The sizes of HindIII DNA fragments are indicated. H, HindIII; B, BamHI. (B) Southern blots of genomic DNA probed with either HindIII5.2-6 or BamHI9-4. Genomic DNA was digested by HindIII. Lane 1, C9-2 (WT); lane 2, 8-88 (ahc); lane 3, 9-39-32 (vc1); lane 4, 24-24-9 (vc2).

The three deletions in ahc, vc1, and vc2 mutants overlap eachother in a region (the 5278-bp HindIII fragment in Fig 3) thatspans a predicted ORF. The ORF starts from position 61,496 bp(start codon) and ends at position 59,292 bp (stop codon) incontig 9a36 (http://www.mips.biochem.mpg.de/proj/neurospora/).An $~$ 4-kbp SacI-HindIII DNA fragment covering the ORF, SAH4-8(Fig 4), was transformed into two vc1 mutants, 9-39-7 (het-c^PAthr-2; vc1 a) and 9-39-10 (het-c^OR pyr-4; vc1 a; Table 1).The introduction of SAH4-8 into 9-39-7 and 9-39-10 did not fullycomplement the profuse conidiation phenotype of the vc1 mutants.To determine whether the introduction of SAH4-8 restored vegetativeincompatibility, heterokaryons were forced between 9-39-7 (SAH4-8)and 9-39-10 (SAH4-8) transformants. These heterokaryons displayedhet-c vegetative incompatibility. We name the ORF required torestore het-c vegetative incompatibility in the vc1 mutant,vib-1.

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Figure 4. DNA sequence of the 4-kbp SacI-HindIII fragment, the predicted amino acid sequence of the vib-1 ORF, and the GC-to-AT transitions in the vib-1(1) and vib-1(2) mutants. The CAAT box, consensus sequence around the start codon CAGTATGGCA, and the polyadenylation site AATAAA are underlined. The NLS sequence is underlined and in boldface type. The KpnI and XhoI sites used for mutational analysis and the HindIII and SacI sites in the 3' UTR region used for deletion constructs are in boldface type. The six GC-to-AT transitions in vib-1(1) (X80-32 and X80-49) are marked by a boldface "A" (the mutant nucleotide) above "G" (the WT nucleotide). The 26 GC-to-AT transition mutations in vib-1(2) (X80-33) are marked by boldface "a" or "t" (the mutant nucleotide) above "G" or "C" (the WT nucleotide; accession number for vib-1: BK000540).

The predicted vib-1 ORF has two introns and three exons andencodes a predicted polypeptide of 670 amino acids (Fig 4).A consensus sequence for translation initiation sites in Neurospora,CAGTATGGCA (EDELMANN and STABEN 1994 ), is present around thepredicted start codon. A CAAT box is located 54 bp upstreamfrom the start codon and a polyadenylation signal, AATAAA, is669 bp downstream from the predicted stop codon. The 3' untranslatedregion (3' UTR) is apparently important for vib-1 function.The introduction of deletion constructs bearing 302 bp (HindIIIsite) or 413 bp (SacI) of the 3' UTR (Fig 4) into the vc1 mutantdoes not restore the capacity for vegetative incompatibility.

vib-1^rip mutants:
Since the deletions in the ahc, vc1, and vc2 mutants could possiblycover additional ORFs besides vib-1, it was necessary to generatevib-1 mutants. Repeat-induced point (RIP) mutation is a naturallymutagenic mechanism in N. crassa (SELKER 1997 ) that acts onduplicated sequences in the genome, such as those introducedby transformation. An $~$ 1-kbp KpnI-XhoI DNA fragment from the5' end of the vib-1 ORF (Fig 4) was transformed into C9-2 (Table 1).A C9-2 (KpnI-XhoI) transformant was crossed with a wild-typestrain 9-1-5 (Table 1). Out of 60 progeny, 3 progeny showinga profuse conidiation pattern were recovered. The conidiationpattern of these progeny was similar to vc1 and vc2 mutantsin plates, race tubes, and slants and their growth rates werealso very similar to vc1 and vc2 mutants (Fig 1).

The $~$ 1-kbp region between KpnI and XhoI in the vib-1 ORF of allthree RIP mutants, X80-32, X80-49, and X80-33, was amplifiedby PCR and cloned. DNA sequencing of the vib-1 fragment in theX80-32 and X80-49 mutants revealed 6 GC-to-AT transitions, whichare typical for sequences that have undergone RIP (SELKER 1997). The mutations occurred in the same sites in the two mutants,suggesting that they came from the same mutagenic event (Fig 4).Three GC-to-AT transition mutations changed Met (55) toIle, Val (227) to Met, and Trp (260) to a stop codon. The other3 GC-to-AT transition mutations occurred in the middle of thefirst intron (after the stop codon). The X80-33 strain contained26 GC-to-AT transition mutations, which caused 15 amino acidchanges and three stop codons. The first stop codon is at Glu(250). Seven amino acid alterations—His (141) to Tyr,Cys (178) to Tyr, Cys (191) to Tyr, Met (200) to Ile, Ala (218)to Val, Val (227) to Ile, and Asp (249) to Asn—occurredin the vib-1 ORF before the first stop codon at amino acid (aa)250 (Fig 4). The vib-1 alleles were named vib-1(1) (X80-32 andX80-49) and vib-1(2) (X80-33).

The ability of the vib-1 mutants to suppress het-c-mediatedvegetative incompatibility was examined by forcing heterokaryonsbetween X80-32 [het-c^OR pyr-4; vib-1(1) A] and X80-49 [het-c^PAthr-2; vib-1(1) A]. The (X80-32 + X80-49) heterokaryons displayeda phenotype that was similar to X80-32 or X80-49 mutants bythemselves (Fig 1; Fig 2A and Fig B). Thus, mutations in vib-1fully relieve growth inhibition and conidiation repression mediatedby het-c vegetative incompatibility.

The vc1 and vc2 mutations were not completely recessive in heterokaryonswith wild-type strains of alternative het-c specificity. Similarto the heterokaryon between a vc1 or vc2 mutant and a wild-typestrain of alternative het-c specificity (Fig 2C), heterokaryonsbetween a wild-type strain and a vib-1(1) mutant of alternativehet-c specificity (X80-32 + Xa-3; Table 1) showed more conidiationand less growth inhibition after 3 days than did wild-type het-cincompatible heterokaryons. Thus, the vib-1(1) mutant phenotypewas indistinguishable from the vc1 and vc2 deletion mutants.

vib-1 mutations alter the pattern of HCD mediated by het-c:
In a het-c incompatible heterokaryon, partial diploid or transformant, $~$ 20–30% of the hyphal compartments have plugged septa andare dead (JACOBSON et al. 1998 ; WU and GLASS 2001 ). The percentageof dead hyphal compartments is fairly uniform across the colonyand has not been associated with any obvious developmental ormorphological feature (such as hyphal fusion junctions). Toassess whether HCD was also suppressed in the vib-1 mutant,we forced a heterokaryon between X80-32 [pyr-4 het-c^OR; vib-1(1)a] and X80-49 [thr-2 het-c^PA; vib-1(1) a] (Table 1) and stainedthe hyphae with the vital dye, Evan's Blue (GAFF and OKONG'O-OGOLA1971 ). Fig 5B&NDASH;D, shows the HCD pattern from a 2-day-oldmycelium of the (X80-32 + X80-49) heterokaryon as compared toa wild-type het-c incompatible heterokaryon (Xa-3 + FGSC 4564, Fig 5A). HCD was not observed in the growth front of the myceliumof the (X80-32 + X80-49) heterokaryon (Fig 5B) in contrast toa wild-type het-c incompatible heterokaryon in which $~$ 20% deadhyphal compartments were observed across the colony (Fig 5A).However, from the growth front toward the inoculation point,HCD rates in the (X80-32 + X80-49) heterokaryon increased to5–10% (Fig 5C and Fig D). The above results indicatethat vib-1(1) mutation does not fully suppress HCD and thatHCD in the vib-1(1) heterokaryons is dependent upon the ageof the mycelium. HCD was also examined in vc1 heterokaryonswith alternative het-c alleles (9-39-10 + 9-39-7; Table 1).The rate and pattern of HCD in the vc1 heterokaryons (whichcontained a deletion covering vib-1) was identical to that ofthe vib-1(1) (X80-32 + X80-49) heterokaryons (data not shown).

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Figure 5. The HCD pattern in heterokaryon [X80-32 (pyr-4 het-c^OR; vib-1(1) A) + X80-49 (thr-2 het-c^PA; vib-1(1) A)] is altered compared to a het-c incompatible heterokaryon. (A) Typical HCD in a 2-day-old het-c incompatible heterokaryon (Xa-3 + FGSC 4564), as observed by staining with the vital dye Evan's blue (GAFF and OKONG'O-OGOLA 1971

). Arrows indicate dead hyphal compartments. Approximately 20% of the hyphal compartments are dead and were distributed randomly across the colony, consistent with previous observations (JACOBSON et al. 1998

; WU and GLASS 2001

). (B–D) HCD in a vib-1(1) heterokaryon (X80-32 + X80-49; Table 1). The 2-day-old vib-1(1) heterokaryon growth distance is $~$ 7 cm. (B) A region 0.5 cm away from the growth front; no HCD was observed. (C) A region $~$ 3 cm away from the growth front. (D) A region $~$ 6 cm away from the growth front; $~$ 5–10% HCD was observed. Bars, 20 µm.

VIB-1 has a predicted nuclear localization sequence and shows similarity to PHOG from Aspergillus nidulans:
Database searches revealed that an internal region of VIB-1(from 157 to 415 aa) was similar to a putative phosphate-nonrepressibleacid phosphatase (An PHOG) from A. nidulans (MACRAE et al. 1993; 41% identity). This region also has a high similarity to apredicted PHOG in Penicillium chrysogenum (Pc PHOG; MARX etal. 1995 ) and to a hypothetical protein, NCU0429.1, in N. crassa(Fig 6). NCU0429.1 is a predicted polypeptide of 719 amino acids(http://www-genome.wi.mit.edu/ annotation/fungi/neurospora/).VIB-1, An PHOG, and Pc PHOG did not show significant similarityto any other predicted proteins in public databases, includingknown phosphatases. A short region of similarity was identifiedbetween VIB-1, An PHOG, and Pc PHOG and a transcription factorfrom Saccharomyces cerevisiae, Ntd80p (23% identity over 143aa, E value 0.003). Ntd80p is required for linking meiosis andsporulation (XU et al. 1995 ; CHU and HERSKOWITZ 1998 ). TheN terminus ( $~$ 100 amino acids) and the C terminus ( $~$ 200 amino acids)of VIB-1 do not show high similarity to any other known or hypotheticalproteins. Computational analysis (http://psort.ims.u-tokyo.ac.jp)showed that VIB-1 has a predicted bipartite nuclear localizationsequence (NLS), RRLQFRIATANNGRRKE, from amino acid position280 to 297. This type of NLS consists of two basic domains separatedby $~$ 10 intervening amino acids (ROBBINS et al. 1991 ). The twobasic domains in VIB-1 NLS are RR and RRK. This putative NLSwas also conserved in the PHOG proteins (Fig 6).

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Figure 6. Alignment of VIB-1 with An PHOG, Pc PHOG, and NCU04729.1. An PHOG is a 330-aa predicted polypeptide from A. nidulans. NCU04729.1 is a predicted 719-aa-long polypeptide in N. crassa (http://www-genome.wi.mit.edu/annotation/fungi/neurospora/) and Pc PHOG is a predicted 593-amino-acid polypeptide from P. chrysogenum. The shaded boxes represent identical amino acids. The predicted NLS is demarcated by a thick line above the conserved sequence.

vib-1 mutants show reduced nonrepressible acid phosphatase activity:
To determine whether vib-1 is a structural gene for nonrepressibleacid phosphatase in N. crassa, native PAGE analysis was usedto detect phosphatase activity in the vib-1 mutants. The stainingmethod employed in this study can detect the activities of bothalkaline and acid phosphatases (DORN 1965 ). As shown in Fig 7,under low-phosphate conditions, four phosphatases were observedfrom the two parental wild-type strains (C9-2 and 9-1-5, lanes1 and 2) and vib-1(1) (X80-32) and vc1 mutants (9-39-10, lanes3 and 4). Under high-phosphate conditions, only nonrepressiblephosphatases were detectable (Fig 7). The activity of the nonrepressibleacid phosphatase (B in Fig 7) is lower in vib-1(1) and vc1mutants compared to that in wild-type strains under both low-and high-phosphate conditions. There were no obvious differencesin A, C, and D in Fig 7 phosphatases between the wild-typestrains and the vib-1(1) and vc1 mutants, except that 9-1-5had lower nonrepressible alkaline phosphatase activity underhigh- phosphate conditions. These data indicate that vib-1 doesnot encode the structural gene for phosphate nonrepressibleacid phosphatase, but may instead encode a positive regulatorof nonrepressible acid phosphatase activity.

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Figure 7. Native gel of phosphatase activity in N. crassa. Fifty micrograms of total protein was loaded per lane. Cultures were grown under low-phosphate or high-phosphate conditions, as described in MATERIALS AND METHODS, prior to protein extraction. The strains used were: lane 1, C9-2 (WT); lane 2, 9-1-5 (WT); lane 3, X80-32 [vib-1(1)]; and lane 4, 9-39-10 (vc1). The predicted phosphatases are A, repressible alkaline phosphatase; B, nonrepressible acid phosphatase; C, nonrepressible alkaline phosphatase; and D, repressible acid phosphatase (HOCHBERG and SARGENT 1973

DISCUSSION

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

In this study and previous work (XIANG et al. 2002 ), we identifiedmutants that suppressed vegetative incompatibility from transformantsthat escaped from vegetative incompatibility mediated by thehet-c locus. By contrast to partial diploids or heterokaryonsthat escaped from vegetative incompatibility mediated by matingtype or het-6 (DELANGE and GRIFFITHS 1975 ; SMITH et al. 1996), the majority of het-c escape transformants (60%) maintainedboth het-c alleles. The compatibility of these escape transformantspresumably was caused by mutations in genes required to mediatevegetative incompatibility or by epigenetic mechanisms. Themutations in these strains could be genetically characterizedbecause they were fertile, in contrast to the near-sterilityof escaped partial diploids used to identify mutations in toland het-6 (VELLANI et al. 1994 ; SMITH et al. 1996 ). Crossesbetween 14 escape transformants and a wild-type strain revealedthree suppressor mutations, ahc, vc1, and vc2. The compatibilityof the other 11 escape transformants might have been causedby mutations closely linked to the het-c locus or by epigeneticmechanisms that silenced het-c during vegetative growth butwhich were not transmitted to progeny (COGONI and MACINO 1999).

The three suppressor mutants all carried independent deletionsin the same region of chromosome V, between lys-2 and ilv-2.The ahc deletion is $~$ 26 kbp and the deletions in vc1 and vc2are $~$ 19 and $~$ 8 kbp, respectively (our unpublished data). It isunclear how these deletions occurred, but the removal of vib-1,a locus responsible for mediating het-c vegetative incompatibility,is probably a major factor involved in their appearance. Hyphaecontaining a nucleus with a deletion or mutation in vib-1 wouldhave a selective advantage for growth and conidiation in anotherwise het-c incompatible colony.

Since the ahc, vc1, and vc2 deletions possibly covered genesin addition to vib-1, we generated vib-1 mutants. The phenotypeof the vib-1 mutants was identical to that of the vc1 and vc2mutants. The distinguishable character of the vc and vib-1 mutantsis the profuse conidiation phenotype, suggesting that vib-1negatively regulates conidiation. A characteristic phenotypicconsequence of vegetative incompatibility in N. crassa is thesuppression of conidiation (MYLYK 1975 ; PERKINS 1975 ). Thesedata suggest that VIB-1-mediated suppression of conidiationis activated or maintained during het-c vegetative incompatibility.

The profuse conidiation pattern of the vib-1 mutants is similarto cpd-1 and cpd-2 (HASUNUMA and SHINOHARA 1985 , HASUNUMAand SHINOHARA 1986 ), cr-1 (see PERKINS et al. 2001 ), andgna-3 (KAYS et al. 2000 ) mutants, all of which have reducedcAMP levels. We speculated that cAMP signaling might be involvedin het-c vegetative incompatibility. The profuse conidiationof a cr-1 mutant (defective in adenylyl cyclase), however, wasfully suppressed in cr-1 het-c^OR/het-c^PA partial diploids (ourunpublished data). These data suggest that het-c vegetativeincompatibility is independent of cAMP signaling. This resultis consistent with data showing that the cAMP pathway is notinvolved in vegetative incompatibility in P. anserina (LOUBRADOUet al. 1999 ).

In addition to the suppression of conidiation, vegetative incompatibilityalso results in growth inhibition and HCD. Mutations in vib-1fully relieve het-c-mediated growth inhibition in heterokaryontests. They cannot, however, fully relieve HCD caused by het-cvegetative incompatibility. In vib-1 or vc1 heterokaryons withalternative het-c alleles, HCD was age dependent and occurredmainly in older hyphae. This pattern is in contrast with theHCD pattern in a wild-type het-c incompatible colony in which $~$ 20% HCD takes place in both young and old mycelia (JACOBSONet al. 1998 ; WU and GLASS 2001 ). The HCD pattern caused byvib-1 mutations is similar to that caused by mod-A mutationsin P. anserina (BERNET et al. 1973 ). It is possible that theremaining level of HCD observed in vib-1 heterokaryons withalternative het-c alleles is caused by NCU0429.1, a proteinsharing high similarity with VIB-1. We are currently mutatingNCU0429.1 to see whether a full relief of HCD in (het-c^PA; vib-1+ het-c^OR; vib-1) heterokaryons will occur.

VIB-1 is a predicted polypeptide of 670 amino acids. It hasbeen annotated to be related to acid phosphatases (Swissprotaccession no. Q05534; MIPS: http://www.mips.biochem.mpg.de/proj/neurospora).The internal 240-amino-acid region of VIB-1 has a high similarityto An PHOG and Pc PHOG, possible phosphate nonrepressible acidphosphatases (nrAPase) in A. nidulans and P. chrysogenum, respectively,but is not similar to any other known phosphatases. The introductionof An phoG into A. nidulans enhanced acid phosphatase activityin a pacG mutant under high-phosphate conditions (MACRAE etal. 1993 ). The pacG mutant reduced activity of nonrepressibleacid phosphatase (CADDICK and ARST 1986 ). An PHOG was thussuggested to be either a nonrepressible acid phosphatase ora regulator of acid phosphatase activity. The Pc phoG gene wascloned by hybridization to An phoG (MARX et al. 1995 ); neitheran An phoG nor a Pc phoG mutant has been described in the literature.Our native gel analysis showed that vib-1 mutants possess allfour phosphatases described in N. crassa (KUO and BLUMENTHAL1961A , KUO and BLUMENTHAL 1961B ; NYC et al. 1966 ; JACOBSet al. 1971 ), including nonrepressible acid phosphatase. Thus,vib-1 is not a structural gene for a nonrepressible acid phosphatase.However, VIB-1 may be a positive regulator of nrAPase becausethe activity of nrAPase was significantly reduced in vib-1(1)and vc1 mutants. VIB-1 has a predicted NLS and could be a nuclearprotein and thus may regulate multiple cellular processes ata transcriptional level. Interestingly, VIB-1 also displayslimited similarity to Ntd80p in S. cerevisiae, a transcriptionalfactor involved in gametogenesis (XU et al. 1995 ; CHU andHERSKOWITZ 1998 ). However, the domain of Ntd80p required forDNA binding to transcriptional targets has not been well defined(E. R. JOLLY, and I. HERSKOWITZ, personal communication).

The relationship between HET-C and VIB-1 is unclear. het-c nullmutants have no phenotype, with the exception that they arefully compatible in heterokaryons with strains with alternativehet-c specificity (SAUPE et al. 1996 ). Non-self-recognitionduring het-c vegetative incompatibility has been associatedwith the formation of a heterocomplex composed of het-c proteinsof alternative specificity (S. SARKAR, G. IYER and N. L. GLASS,unpublished data). It is possible that VIB-1 is required forformation of a HET-C heterocomplex and thus that the vib-1 mutantsuppresses het-c vegetative incompatibility because the HET-Cheterocomplex fails to form. Alternatively, the HET-C heterocomplexmay form in the vib-1 mutant, but vegetative incompatibilityis not triggered. Experiments are currently underway to determinethe effect of the vib-1 mutation on HET-C heterocomplex formation.

We conclude that vib-1 is a gene involved in multiple cellularprocesses. In addition to vegetative incompatibility, it isalso implicated in the regulation of conidiation and nrAPase.What is the relationship between het-c vegetative incompatibilityand nrAPase? The first possibility is that VIB-1 regulates multiplecellular processes, such as nrAPase production, conidiation,and vegetative incompatibility, and thus there is no causalconnection between vegetative incompatibility and nrAPase. Thesecond possibility is that VIB-1 regulates nrAPase, which isrequired to mediate vegetative incompatibility. In N. crassa,it has been speculated that nrAPase participates in metaboliccontrol systems rather than in phosphate uptake (KUO and HERSKOWITZ1961b). Thus, nrAPase may be involved in the regulation of certaincellular processes in N. crassa, including vegetative incompatibility.We are currently conducting experiments to distinguish thesetwo possibilities.

ACKNOWLEDGMENTS

We thank Drs. Robert Metzenberg, Patrick Shiu, and JenniferWu for technical help and Dr. George Haughn for helpful suggestions.We thank members of the Glass laboratory for critical readingof this manuscript. This work was funded by a National Institutesof Health grant (GM-60468-01) to N.L.G.

Manuscript received April 8, 2002; Accepted for publication June 10, 2002.

LITERATURE CITED

TOP
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DISCUSSION
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