©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
Identification and Characterization of a Gene Encoding Phospholipase D Activity in Yeast (*)

(Received for publication, November 1, 1995; and in revised form, December 7, 1995)

Michal Waksman (1) Yona Eli (1) Mordechai Liscovitch (1) Jeffrey E. Gerst (2)(§)

From the  (1)Department of Biological Regulation and (2)Department of Molecular Genetics, Weizmann Institute of Science, Rehovot 76100, Israel

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

We have identified an open reading frame on chromosome XI of the yeast, Saccharomyces cerevisiae, as encoding a protein with phospholipase D (PLD) activity. We have named this open reading frame, PLD1, and show that yeast bearing a disruption in this gene are unable to catalyze the hydrolysis of phosphatidylcholine. PLD1 encodes a hypothetical protein of 1683 amino acids and has a predicted molecular mass of 195 kDa. Yeast bearing disruptions at the PLD1 locus are morphologically normal and grow vegetatively like wild-type cells. In contrast, homozygous Deltapld1 diploid cells are unable to sporulate and do not produce asci under conditions that induce meiosis and sporulation in wild-type cells. Thus, PLD1 is likely to be essential for the meiotic cycle in yeast cells.

This is the first identification of a eukaryotic, non-plant, phosphatidylcholine-hydrolyzing phospholipase D gene. Because the biological role of PLD is not well understood, we expect that Deltapld1 yeast will become a useful tool for the characterization of PLD functions as well as for the identification of mammalian PLD homologs.


INTRODUCTION

Phospholipase D activity has been identified in a wide variety of cell types and organisms from bacteria(1) , yeast(2) , plants(3) , and mammals (reviewed in (4) and (5) ). PLD acts to catalyze the hydrolysis of certain phospholipids, i.e. catalyzing the hydrolysis of phosphatidylcholine (PC) (^1)to yield phosphatidic acid (PA) and choline. PA, itself, is thought to act as an intracellular second messenger in PLD-induced signaling processes (reviewed in (5) ) and may also be involved in regulating the synthesis of phosphatidylinositol 4,5-bisphosphate (PIP(2)) (6) .

Activation of PLD in mammals occurs via known receptor-mediated mechanisms (reviewed in (5) ), and evidence exists for the involvement of protein kinase C(5, 7) , heterotrimeric GTP-binding (G) proteins (reviewed in (5) and (8) ), and small G proteins of the ARF and Rho families in its activation(9, 10, 11, 12) . Two distinct activation requirements for mammalian PLD have been described: one type of enzymatic activity is GTP- and ARF-dependent, while another is oleate-dependent(13) . However, both types of enzymatic activities can be stimulated by PIP(2)(13, 14) . Interestingly, recent studies have shown that PIP(2) biosynthesis, itself, is a direct prerequisite for PLD activation(15) , which suggests that PIP(2) is a co-factor of PLD.

Recent work has implicated the activation of both phosphoinositide (PI) metabolism and ARF as necessary steps for the intracellular trafficking of membrane-bound compartments (reviewed in (16, 17, 18) ). Since PLD activity in mammals may be activated by either ARF or PIP(2), it is intriguing to think that PLD could play an important role in mediating membrane trafficking. Yet, despite the wealth of information concerning the biochemical properties of PLD, little is known about the structural and molecular properties of the enzyme(s), while even less is known about its biological role. To date, the only published sequence for a protein from eukaryotes having PC-specific PLD activity is from plants(3) , and its role in either cell signaling or membrane trafficking remains virtually unknown.

Here we describe the identification and characterization of a gene encoding a PLD from yeast. We show that the yeast enzyme is homologous to plant PLD and shares some homology with a bacterial phosphatidyltransferase. Disruption of the PLD1 gene in yeast has no effects upon cell growth and morphology during vegetative growth but is likely to be required for meiosis and sporulation.


EXPERIMENTAL PROCEDURES

Chemicals

PIP(2) was obtained from Sigma. 1-Palmitoyl-2-[6-N-(7-nitrobenzo-2-o-1,3-diazol-4-yl)amino]caproyl-phosphatidylcholine (C(6)-NBD-PC) was purchased from Avanti Polar Lipids.

DNA Manipulations

DNA restriction endonucleases, Taq polymerase, and T4 DNA ligase were used as recommended by the suppliers (Boehringer Mannheim, MBI Fermentas). Molecular cloning techniques were performed as described by Sambrook et al.(19) .

Media and Genetic Manipulations

Yeast were maintained on standard growth media containing 2% glucose as a carbon source. Amino acid-rich medium (YPD (yeast extract and Bactopeptone containing 2% dextrose)) and YP (yeast extract and Bactopeptone), synthetic minimal medium (SC), and SC drop-out medium, lacking an essential amino acid or nucleotide base, were used. Drop-out medium was used to maintain plasmid selection. Media were prepared according to Rose et al.(20) . SC complete and drop-out media consisted of 0.7% yeast nitrogen base supplemented with the appropriate auxotrophic requirements. Other growth media included: YPA (YP containing 0.05% glucose and 2% potassium acetate); YPEG (YP containing 2% ethanol and 2% glycerol); and YPG (YP containing 3.5% galactose). Standard methods were used for the introduction of DNA into the various yeast strains, the preparation of genomic DNA, and for tetrad dissection (20) . Escherichia coli strain XL-1 blue was used for plasmid transformations and plasmid DNA preparations.

Yeast Strains

Disruptions of PLD1 were made in wild-type strains JC1 (Matalpha ade8 can1 his3 leu2 lys2 trp1 ura3) (21) and JC2 (Mata ade8 can1 his3 leu2 lys2 trp1 ura3). Deltapld1 strains created included: PLDDelta-1 (Matalpha ade8 can1 leu2 lys2 trp1 ura3 Deltapld1::HIS3); PLDDelta-2 (Mata ade8 can1 leu2 lys2 trp1 ura3 Deltapld1::HIS3); PLDDeltaFS-1 (Matalpha ade8 can1 leu2 lys2 trp1 ura3 Deltapld1::HIS3); and PLDDeltaFS-2 (Mata ade8 can1 leu2 lys2 trp1 ura3 Deltapld1::HIS3).

Plasmids

Cosmid pEKGO13, which contains a genomic fragment from chromosome XI in vector pWE15, was a gift from A. Urrestarazu (Universite Libre de Bruxelles). This cosmid contains 36 kb, which maps to the small arm of chromosome XI and encompasses mapped genes spo14 and tif1. Disruption constructs for PLD1 were created by subcloning a 5.1-kb EcoRI/XhoI fragment containing the coding region of PLD1 beginning at bp 837 and ending at bp +912 downstream of the termination codon into the EcoRI/SalI sites of pUC118 to yield pPLD. This plasmid was then digested with the SalI endonuclease to release an 1153-bp fragment (bp 3237-4390), which is thought to encode part of the catalytic domain of Pld1 (see Fig. 1, homology boxes 6 and 7) and was blunt-ended using standard techniques. A blunt-ended BamHI-cut 1.7-kb fragment encoding the HIS3 auxotrophic marker was then subcloned in to yield plasmid pPLD::HIS3. To create a frameshift mutation near the initiation codon of Pld1, plasmid pDeltaPLD::HIS3 was digested with SacI (bp 871), filled in using the Klenow fragment of DNA polymerase, and religated to yield a frameshift disruption plasmid, pDeltaPLDFS::HIS3. All plasmids were verified by restriction mapping.


Figure 1: Homologous regions of ORF YKR031c and plant PLD. The diagram in A illustrates ORF YKR031c. Numbers above the diagram indicate those regions (marked boxes) ranging between 11 and 42 amino acids that are highly homologous to regions of plant PLD. Beneath each box is the percentage identity shared between residues of YKR031c and plant PLD within that designated region. The corresponding number of amino acids for each given region is: 1-25, 2-20, 3-19, 4-42, 5-28, 6-11, 7-37, and 8-24, respectively. B shows sequence comparisons between plant PLD and YKR031c contained within boxes 4, 5, and 7. An additional comparison between YKR031c and phosphatidylserine synthase from E. coli (PSS) is shown. Numbers correspond to amino acid sequence of the proteins; identities are marked with a vertical bar, and conserved residues are marked with a colon.



To create disruptions of PLD1 in yeast, plasmids pDeltaPLD::HIS3 and pDeltaPLDFS::HIS3 were digested with EcoRI and SphI to release fragments containing the disrupted PLD1 gene. These were transformed into yeast cells using standard procedures to create the strains described above. All disruptions were verified by Southern analysis.

Phospholipase D Assay

Total cell lysates from yeast grown at log phase were prepared as described previously(22) , except that the lysis buffer contained 35 mM HEPES pH 7.0, with no added detergent. Lysates were cleared by low speed centrifugation (16,000 times g for 0.25 min) to remove nuclei and cell wall debris. Cell lysates were flash frozen and stored at -70 °C.

The hydrolysis of C(6)-NBD-PC in lysates was monitored by the production of PA, essentially as described by Danin et al. (23) . Briefly, the reaction mixture contained 0.3 mg/ml protein, 35 mM HEPES pH 7.2, 150 mM NaCl, 0.4 mM C(6)-NBD-PC, and 4 mol % PIP(2). Reaction volume was 120 µl, and the reactions were incubated at 30 °C for 30 min. Transphosphatidylation assays contained between 0 and 500 mM primary alcohol as substrate. The assays were terminated by chloroform/methanol/HCl extraction (100:100;0.6), and the phospholipid products were separated by thin layer chromatography (TLC), as described(23) . Fluorescent phospholipids were visualized by UV illumination, scraped from TLC plates, methanol-extracted, and counted in a fluorimeter (excitation at 468 nm; emission at 520 nm). Results are expressed as the average of two duplicate samples measured in arbitrary fluorescence units.


RESULTS

Identification of a Yeast Homolog of Plant PLD

Recent identification of a PC-specific PLD from plants allowed us to screen the National Center for Biotechnology Information (NCBI) data base for sequences having direct homology. Interestingly, an ORF from Saccharomyces cerevisiae that encodes a hypothetical protein of 1683 amino acids was found to have significant homology to certain regions of plant PLD when searched using the BLAST algorithmic program (24) . This ORF was identified by the yeast genome sequencing project (ORF YKR031c) and maps to the short arm of chromosome XI by the GCN3-DAL80 intergenic region and near the previously mapped spo14 and tif1 genes.

Sequence comparison between the proteins showed that they had low overall homology. However, at least eight specific regions of 11-42 amino acids in length were found to be highly homologous, ranging from 50 to 76% (Fig. 1). The percentage of shared residues in these regions varied between 20 and 62% (Fig. 1). One region, in particular, was also identified as having homology to a phosphatidylserine synthase from bacteria (Fig. 1, homology box 7). Thus, ORF YKR031c seemed a likely candidate for a yeast protein having PLD activity and was tentatively renamed PLD1.

Identification of ORF YKR031c as a Phospholipase D

In order to verify that this ORF encodes a yeast PLD homolog, we constructed haploid and diploid yeast strains lacking PLD1 (see ``Experimental Procedures''). Yeast-bearing disruptions in PLD1 were found to be morphologically normal and grew at rates similar to wild-type cells grown under vegetative conditions (data not shown). Moreover, these Deltapld1 cells were found to be temperature-resistant like wild-type cells (data not shown).

In order to verify that Deltapld1 cells lack PLD activity, we performed PLD assays in vitro on yeast cell lysates, using the fluorescent PC analog, C(6)-NBD-PC, as substrate. Wild-type cells of either mating type were found to have significant levels of PLD activity, as judged by PA production (Fig. 2). In contrast, Deltapld1 cells were found to have no detectable PLD activity, indicating that the disruption of PLD1 destroys the protein responsible for PLD function. Thus, the PLD1 gene product (Pld1) is likely to confer PLD-like activity.


Figure 2: Measurement of PLD activity in wild-type cells and Deltapld1 disruption strains. The production of PA from fluorescent-labeled phosphatidylcholine (C(6)-NBD-PC) in lysates prepared from wild-type (WT) and Deltapld1 cells was performed (see ``Experimental Procedures''). Included in the assay were EGTA (5 mM), EDTA (1 mM), and octyl glucoside (0.2 mM). PA production is measured at an emission wavelength of 520 nm and given in fluorescence units. A shows a photograph of the fluorescence-based emission taken of the samples chromatographed on TLC plates. B represents a histogram of the data shown in A. Lanes 1 and 20 indicate PA production in the absence of added protein. Lanes 2-4 and 11-13 indicate PA production in membrane preparations from JC1 and JC2 wild-type cells, respectively. Lanes 5-7 indicate PA production in Deltapld1 strain PLDDelta-1, while lanes 8-10 indicate PA production in Deltapld1 strain PLDDeltaFS-1. Lanes 14-16 indicate PA production in pld1 strain PLDDelta-2, while lanes 17-19 indicate PA production in Deltapld1 strain PLDDeltaFS-2. Lane 21 contains a standard for phosphatidic acid.



Characterization of Pld1 Activity

A previous study has characterized biochemically PLD activity in yeast(2) . This activity localizes primarily to membrane fractions and was found to be both PC-specific and capable of utilizing short chain alcohols in the transphosphatidylation reaction(2) . Moreover, the rank order of straight and branched chain alcohols in the transphosphatidylation reaction was similar to that already described for mammalian cell PLDs. Finally, it was shown that maximal PLD activity in yeast could be induced in a cycloheximide-independent manner by shifting cells to sporulation-inducing medium, which contains acetate(2) .

To verify that the activity of the PLD1 gene product is similar to that described previously, we have characterized PLD activity in wild-type and Deltapld1 cells (Fig. 3). We first examined the effect of primary alcohol addition upon PA production and alcohol transphosphatidylation in haploid cells. We found that an increase in alcohol chain length resulted in a decrease in the overall activity of the enzyme, which was characterized by both a decrease in PA formation and an increase in phosphatidyl alcohol production (Fig. 3A). Next, we examined the effect of various agents and carbon sources upon PLD activity. The addition of chelators of divalent metal cations or oleate resulted in a significant decrease in PLD activity (Fig. 3A). Likewise, the omission of PIP(2) led to a substantial decrease (>65%) in activity (Fig. 3A). Thus, the PLD activity examined here is highly similar to that described previously (2) and is similar to the oleate-independent PLD from mammals(13) .


Figure 3: Characterization of yeast PLD activity. PLD activity (PA production) was assayed under different conditions. A, the ability of straight chain alcohols to serve as substrates for the transphosphatidylation reaction is shown in lanes 1-4. PA production was assayed with the addition of 0.5 M primary alcohol (e.g. ethanol (Eth), propanol (Prop), and butanol (But)) and is shown as a solid bar. In addition, the amount of phosphatidyl alcohol produced was also assayed and is shown above as a hatched bar. The effect of divalent cation chelators (EGTA/EDTA) upon PA production is shown in lane 5, while the effects of oleate addition (60 mol%, lane 6) or the omission of PIP(2) from the assay (lane 7) is also given. The amount of PA/phosphatidyl alcohol production is normalized (in percent) to the amount of activity generated under standard assay conditions in the presence of PIP(2). Activity was assayed in lysates prepared from JC1 wild-type yeast. B, the effect upon PLD activity of growing cells on different carbon sources. Wild-type yeast (JC2) were grown for 6 h on a variety of rich media containing different carbon sources (lane 1, glucose (YPD); lane 2, acetate (YPA); lane 3, ethanol/glycerol (YPEG); and lane 4, galactose (YPG)). PA production in cell lysates was assayed as described (see ``Experimental Procedures''). In a different experiment, homozygous Deltapld1::HIS3/Deltapld1::HIS3 (PLDDeltaFS-1 times PLDDeltaFS-2 cells) and heterozygous Deltapld1::HIS3/PLD1 (PLDDeltaFS-1 times JC2) cells were assayed for PA production when shifted to acetate-containing medium (YPA) (lanes 6 and 8) for 2 h or maintained continually on glucose (YPD) (lanes 5 and 7). The activities for these representative experiments are listed in arbitrary fluorescence units.



In contrast, growing cells in the presence of non-fermentable carbon sources, such as acetate and ethanol/glycerol, or in the presence of galactose resulted in an increase in PLD activity over cells maintained continually in glucose. Thus, the yeast enzyme may be under partial glucose-repressible control (Fig. 3B).

Since yeast PLD is stimulated in the presence of acetate-containing medium (this study and (2) ), we examined whether PLD activity is increased in homozygous Deltapld1::HIS3/Deltapld1::HIS3 and heterozygous Deltapld1::HIS3/PLD1 cells shifted from glucose-containing medium to acetate-containing medium (sporulation conditions). Cells bearing homozygous disruptions in PLD1 showed little basal activity when grown in glucose-containing medium or when shifted to acetate-containing medium. In contrast, heterozygous Deltapld1::HIS3/PLD1 diploid cells showed a strong time-dependent induction of PLD activity that peaked within 2 h of shifting the cells to acetate-containing medium (Fig. 3B and data not shown). Thus, PLD activity is induced under sporulation conditions in a PLD1-dependent fashion.

The stimulation of PLD activity upon transfer to acetate-containing medium suggested to us that a functional PLD might be required for sporulation in yeast. Indeed, diploid yeast bearing homozygous disruptions of PLD1 (Deltapld1::HIS3/ Deltapld1::HIS3) were found to be unable to undergo sporulation to yield asci under conditions by which wild-type cells are known to sporulate (data not shown). Thus, there appears to be a requirement for PLD1 in the sporulation of yeast cells.


DISCUSSION

We have identified a yeast protein that confers PLD activity to yeast cell lysates. The gene encoding this activity, PLD1, localizes to the GCN3-DAL80 intergenic region of the short arm of chromosome XI and is the region that the spo14 sporulation mutation maps to. Our results indicate that PLD1 encodes a PC-hydrolyzing PLD that confers the significant, if not total proportion, of PLD catalytic activity in yeast cells. Moreover, this activity is stimulated during sporulation conditions and is similar in requirements to that described previously by Ella et al. (2) . In addition, we have demonstrated that yeast Pld1 is stimulated by PIP(2) like mammalian PLD(14) .

Although the true role of PLD1 is not yet known, strong evidence links PLD function to meiosis and sporulation in yeast cells. First, PLD1 activity is stimulated during the shift to sporulation-inducing medium (this study and (2) ). Second, Deltapld1 cells fail to undergo sporulation. Third, while this manuscript was in preparation, the sequence of SPO14 was deposited into the NCBI data base (accession number L46807) and although it was not identified as having PLD activity, we and others have now identified it as being allelic to PLD1. (^2)Thus, PLD activity appears necessary for yeast cells to complete the meiotic cycle.

When diploid yeast are deprived of nitrogen and fermentable carbon sources they enter a meiotic cycle that leads to the development of four haploid nuclei. These nuclei are later enveloped by a membranous spore wall that arises from the coalescence of vesicles at the spindle pole (reviewed in (25) ). The spore wall consists of four layers, including at least two spore-specific layers that are induced only during the meiotic cycle. SPO14 was previously identified as a sporulation-specific gene that is required for the commitment to meiotic development as well as for meiotic segregation and spore formation(26) . Cells bearing the spo14 mutation are defective in sporulation but can return to mitotic division even from the late stages (i.e. tetraploid stage) of meiotic development(27) . In all likelihood, then, Spo14/Pld1 may be a critical component of the final stage of the meiotic cycle, spore wall assembly.

Converging lines of evidence have implicated PLD function with PI metabolism and membrane trafficking in mammals(17) . Activation of PLD by ARF, which itself acts to recruit cytosolic coat proteins to newly forming vesicles in the Golgi (reviewed in (18) ), may be an important mechanism for generating PA and altering the lipid environment on membranes destined to undergo fusion(17) . However, PLD activation may also lead to PIP(2) production(17) , which could have profound effects upon both PI metabolism and signaling via PI-mediated signaling cascades, in addition to affecting the lipid environment of membranes. Although this work is still in its infancy, yeast may prove to be an ideal system in which to assay the role of PLD upon PI metabolism, as well as in cell signaling and membrane trafficking. Interestingly, our work already demonstrates that Pld1 activity is not necessary for vegetative cell growth, which implies that membrane trafficking processes like secretion are not prominently affected. Thus, we predict that Pld1 function is not likely to be required for the anterograde trafficking of secreted essential proteins, although it could play a role in other trafficking steps.


FOOTNOTES

*
This work was supported by grants from the Israel Science Foundation (to M. L.) and the Forchheimer Center for Molecular Genetics (to J. E. G.). The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
Supported by a Yigal Allon fellowship and incumbent of the H. Kaplan career development chair for cancer research. To whom reprint requests should be addressed. Tel.: 972-8-342106; Fax: 972-8-344108; :lvjeff{at}weizmann.weizmann.ac.il.

(^1)
The abbreviations used are: PC, phosphatidylcholine; ARF, ADP-ribosylation factor; C(6)-NBD-PC, 1-palmitoyl-2-[6-N-(7-nitrobenzo-2-o-1,3-diazol-4-yl)amino]caproyl-phosphatidylcholine; ORF, open reading frame; PA, phosphatidic acid; PC, phosphatidylcholine; PI, phosphoinositide; PIP(2), phosphatidylinositol 4,5-bisphosphate; PLD, phospholipase D; kb, kilobase(s); bp, base pair(s).

(^2)
This study and J. Engebrecht, personal communication.


ACKNOWLEDGEMENTS

We thank Dr. A. Urrestarazu for the gifts of cosmid and bacteria. We are also grateful to Drs. J. Engebrecht and A. Morris for sharing unpublished results.

Note Added in Proof-After this work was accepted, a paper describing the identification of a human PLD gene was published (Hammond, S. M., Altshuller, Y. M., Sung, T-C., Rudge, S. A., Rose, K., Engebrecht, J., Morris, A. J., and Frohman, M. A.(1995) J. Biol. Chem.270, 29640-29643). This gene is highly homologous to [Abstract/Full Text] yeast PLD1.


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