- Email: [email protected]
Vectors for inserting selectable markers in vector arms and human DNA inserts of yeast artificial chromosomes (YACs)
Gene, 103 (1991) 53-59 0 1991 Elsevier Science
GENE
Publishers
B.V. All rights reserved.
53
0378-l 119/91/$03.50
05026
Vectors for inserting selectable markers in vector arms and human DNA inserts of yeast artificial chromosomes (YACs) (Homologous
recombination;
plasmid;
neomycin
resistance;
LYS2 gene; LI element;
thymidine
kinase;
recombinant
DNA)
Anand K. Srivastava and David Schlessinger Department of Molecular Microbiology and Center for Genetics in Medicine, Washington UniversitySchool of Medicine, St. Louis, MO 63110 (U.S.A.) Received by G.N. Gussin: 17 December Revised: 8 March 1991 Accepted: 13 March 1991
1990
SUMMARY
To facilitate studies of gene expression and homologous recombination, plasmids have been developed which permit the insertion of neomycin resistance-encoding gene (NmR) into either the human DNA insert or the vector arm of a yeast artificial chromosome (YAC). To integrate into the YAC arm, the plasmid pRV1 contains a LYS2 (encoding a-aminoadipate reductase) gene for selection in the yeast host, and a NmR gene for subsequent selection after transfection of mammalian cells. These two sequences are bracketed by fragments of the URA3 gene (encoding orotidine-5’-phosphate decarboxylase) that can disrupt the URA3 gene in the YAC arm by homologous recombination in yeast. To integrate a selectable marker into the insert, the plasmid pRV2 contains a NmR gene and an intact copy of the URA3 gene, bracketed by segments of an LI (LINES) repetitive element. In this case, the vector has been designed for use with YACs that have already been fitted in the vector arm with a different marker (i.e., TK) that has disrupted the URA3 gene in the vector arm. Selection is for the restoration of URA3 gene activity attendant on recombination into an Ll element in the YAC insert. Use of the vectors is illustrated with a YAC clone containing ribosomal DNA.
Transfection studies of DNA constructs have become a standard way to examine the function of gene sequences. The size of DNA fragments that can be accommodated in traditional bacterial and phage vectors has been limited, however. Consequently, for many genes, it was difficult to
achieve constructs with the signals required for a number of regulatory phenomena, including tissue-specific expression and mRNA metabolism (DeChiara et al., 1990; Reid et al., 1990). The introduction of vectors in which large DNA inserts can be maintained has provided potential reagents for the study of even large genes. The YACs (Burke et al., 1987)
Correspondence to: Dr. D. Schlessinger, Department of Molecular Microbiology, Washington University School of Medicine, St. Louis, MO
LYS2, gene encoding
63110 (U.S.A.)
gene encoding
INTRODUCTION
Tel. (314)362-2744;
Fax (314)362-1232.
cation; encoding
Abbreviations: aa, amino acid(s); Ap, ampicillin; bp, base pair(s); CHEF, contour-clamped hexagonal electrophoresis; EtdBr, ethidium bromide;
Ll (LINES), large interspersed
kb, kilobase(
a-aminoadipate
Nm resistance;
PFGE,
pulsed-field
nt, nucleotide(s); gel electrophoresis;
TK; TK, thymidine
ribosylanthranilate phate decarboxylase;
reductase;
isomerase;
kinase;
repeated
sequence(s);
Nm, neomycin; r, ribosomal;
TRPI, gene encoding
URA3, gene encoding
YAC, yeast artificial
NmR,
on’, origin of DNA repliTK, gene phospho-
orotidine-5’-phos-
chromosome.
54 in particular, can be used to clone most genes in complete form and in normal sequence context. For example, YAC cloning has permitted the recovery of intact genes, including factor VIII (Abidi et al., 1990) factor IX (Brownstein et al., 1989) glucose-6-phosphate dehydrogenase (G6PD gene; D’Urso et al., 1990) and glycineamide ribonucleotide transformylase (GART gene; Gnirke et al., 1990); the last two have been shown to produce active enzyme from YACs upon transfection of mammalian cells (D’Urso et al., 1990; Gnirke et al., 1990). To investigate the expression and fate of YACs in detail, it is necessary to establish them stably in recipient cells. A selective marker can be part of the YAC vector when a library is constructed (Traver et al., 1989); but a large number of currently available YACs contain no such marker including the original and still widely used pYAC4 (Burke et al., 1987). For those, modification of the existing YAC with appropriate markers, a process that has been called ‘retrofitting’, is indispensible. We have reported one vector (TKLU2) which can be used to introduce the selectable TK gene into the vector arm of a YAC (Eliceiri et al., 1991). This facilitates the subsequent selection of TK-deficient mammalian cells that have been stably transformed with the modified YAC (Eliceiri et al., 1991). Use of the TK gene as a selective marker is restricted to cell lines deficient for the gene. Here we describe two additional vectors, pRV1 and pRV2, which extend the use of such a system to mammalian cells in general. Both plasmids contain the NmR gene, a marker selectable in mammalian cells, and can introduce it, respectively, into a dispensible portion of a YAC (the vector arm) or into the insert DNA of a YAC. Adding Nm R to the vector arm with pRV 1 permits direct transfection studies. With a similar aim, NmR has been introduced into a repetitive sequence (Ah) in the human insert of a YAC (Pavan et al., 1990). In contrast, rather than fitting a YAC directly with the NmR gene in the insert, pRV2 is designed to be used in a second step with YACs that have already been retrofitted with the TK gene in the vector arm. As a result of the successive use of the two vectors TKLU2 and pRV2, YACs are recovered that permit one to select for the NmR marker in the insert and against the TK marker in the arm. This imitates in YACs the positive-negative selection system developed by Mansour et al. (1988) (see Thomas and Capecchi, 1990) to promote gene alteration by a homologous copy in a 2 phage.
obviate the need to make YACs with vectors that commit one to the use of only a particular selective marker, and free one from the dependence on available restriction sites for recombinant DNA manipulations. (a) Retrofitting YAC vectors arms with the NmR gene In construct pRV1 (Fig. 1) the NmR and LYS2 genes were inserted at a unique site within the URA3 gene. Construction was begun by subcloning a 3.7-kb EcoRI-BamHI fragment of plasmid pdBPV-MMTneo (Law et al., 1983) containing the NmR gene, between the EcoRI and BamHI sites of pUC18 (Yanisch-Perron et al., 1985). The resulting plasmid, pNm, was linearized with BamHI. The ends were made flush using the Klenow fragment of E. co/i DNA polymerase I and dNTPs, and the terminal phosphates were then removed by calf thymus alkaline phosphatase (Maniatis et al., 1982). A 5.2-kb EcoRI-Hind111 fragment of plasmid YIp333 (Eibel and Philippsen, 1983) containing the LYS2 gene, which had also been rendered blunt-ended
A
B kb 450350 -
I
Nlll
Fig. 1. Targeting ofthe Nmamarker into a YAC vector arm. (A) Diagram of retrofitting vector pRV1. Only unique restriction sites are shown. (B) PFGE
analysis
were grown
lysine
described
of seven clones (Trp + Ura-
in synthetic
liquid medium
and tryptophan,
low-melting-agarose AND DISCUSSION
blocks
gel shows
and
Lys2 + ). Transformants
supplemented
DNA
yeast
DNA transferred
with aa mixture
was immobilized
and fractionated
in a CHEF
by Carle and Olson (1985). A 1% agarose
TBE buffer with switching
The highly recombinogenic nature of yeast facilitates the modification of resident YACs to incorporate markers that can promote their retention in mammalian cells by selection. Standard techniques of gene disruption and insertion
3456769
7
lacking RESULTS
2 1 .
in 0.5”;
apparatus
as
gel was run in 0.5X
time of 15 s to 30 s for 20 h. The EtdBr-stained
chromosomes
and YACs.
to a nylon membrane
(C)Autoradiogram
(Sureblot,
Oncor)
of the
from the gel
in panel B and hybridized to NmR probe DNA. Lanes 1-3 and 5-8, YACs; lane 9, parental YAC; lane 4, marker of concatamerized I genomes. Arrow
indicates
the position
of YACs.
55 as above, was then ligated to the linear blunt-ended plasmid. The EcoRI-Hind111
fragment
of the plasmid
pNm
bearing the
fused NmR and LYS2 genes was made blunt-ended as described above, repurified, and inserted at a unique Stul site within the URA3 gene [contained on the Hind111 restriction fragment of plasmid YEP24; Botstein et al. (1978) and cloned into the Hind111 site of pUCl8 (Yanisch-Perron et al., 1985)]. Digestion of plasmid pRV1 with Hind111 (Fig. 1A) released a 9.5-kb fragment containing the LYS2 and Nm R genes between segments of the yeast URA3 gene.
513-bp
HinfI-SnaBI
fragment
portion
of a human
Ll
repeat
containing
a 3’-conserved
was isolated
from pCD
KpnI-8 (Scott et al., 1987) and cloned into the SmaI site of pUCl8.) Since LI elements are not present in yeast DNA, LI in the vector should selectively recombine into the Ll of the human DNA insert of YACs. LI have several advantages as a target for the introduction of selectable markers in the human DNA inserts of YACs. These include: (i) Their frequency. LI occurs about once every 50 kb in total human DNA (Singer and Skowronski, 1985) and would therefore likely occur several times in typical YACs
Integrative disruption of the URA3 gene in the YAC arm by this fragment produced recombinants that had become
of 100 to 600 kb. Thus, the selective marker can be intro-
Lys’ Ura in yeast and contained the Nm R gene. In pilot experiments, pRV1 was used to introduce
duced at a fixed number of sites, making it flexible enough to yield a probable insertion at a site useful for a variety of
the
NmR marker into several YAC clones. For example, yeast carrying yA16G4, a YAC clone containing human rDNA (Labella and Schlessinger, 1989) was transformed with 0.25, 0.5 and 1.0 pg of gel-purified pRV1 fragment by the spheroplasting procedure (Burke et al., 1987). From several experiments, 96 colonies were selected for growth in the absence of lysine (due to the L YS2 gene in the right arm of the YAC) and tryptophan (due to the TRPI gene in the left arm of the YAC). Of the 96, 69 were also Ura- (the other strains may have undergone recombination into the already inactive chromosomal URA3 gene, and thus retained an intact homologue in the YAC arm). DNA from seven randomly chosen transformants was fractionated by PFGE (Carle and Olson, 1985) (Fig. 1B). The normal distribution of yeast chromosomes in the range of 200 to 500 kb is seen in the EtdBr-stained gel, along with the modified YACs. Five of the seven contained a 160-kb YAC, as expected (lanes 3 and 5-8); lane 9 shows the smaller parental YAC before modification. The DNA was transferred to a nylon membrane and analyzed by hybridization with probes that included a 3.7-kb EcoRI-BamHI fragment of pdBPVMMTneo containing the NmR gene (Law et al., 1985) and labeled using the random primer method of Feinberg and Vogelstein (1983). Fig. 1C indicates that the five YACs of the anticipated size also contained NmR gene sequences. Insertion of the NmR gene into the YAC was also verified by analysis of the products of restriction enzyme digestion (data not shown). (b) Adapting YACs to promote homologous in human cells
recombination
(1) Principles of using Ll element To introduce the mammalian selectable marker (NmR) into the human DNA insert of a YAC, we capitalized on the occurrence of repetitive LINES (LZ) elements (Scott et al., 1987) in human DNA. Vector pRV2 contains a NmR cassette and a URA3 gene between human LI repeats. (A
purposes, but infrequent enough to be relatively easy to map the site of insertion in the YAC. (ii) Their constancy. The part of Ll outside the portion used varies almost as much as Ah sequences (Deininger, 1989) and can be ofhighly variable length (Hutchison et al., 1989); but the segment employed (517 nt at the 3’ end) is highly conserved in the range of Ll in the human genome. This makes it highly likely that the transforming fragment will be inserted at a comparable site in the repetitive sequence in all cases, and with a comparable chance of recombining with every Ll element. (2) Procedures The vector pRV2 is designed to be used in a two-step procedure (Fig. 2A) to put a positive selectable marker into the insert of a YAC and a negative selectable marker into the vector arm. In step one, using vector TKLU2 (Eliceiri et al., 1991), a YAC was first modified by insertion of the TK gene into the URA3 gene in the YAC vector arm. Yeast cells carrying a YAC with the resultant Trp + Ura- Lys + phenotype were selected and the NmR gene was inserted into their human DNA moiety using the vector pRV2. The final recombinants were Trp’ Lys’ and had the Ura+ phenotype restored (Fig. 2A). This strategy was tested on the same YAC (yAl6G4) used in Fig. 1. The presence of LI in this YAC had already been confirmed, making it feasible to insert DNA at those sites. Yeast cells containing the YAC were transformed with the Hind111 restriction fragment of plasmid TKLU2 containing the TK and LYS2 genes. Insertion of the TK gene into the vector arm of several of the Trp + Ura- Lys + YACs was verified by restriction analysis, and by hybridization with a probe that included a 2040-bp PvuII fragment of plasmid TK321 (Majors and Varmus, 1983) containing the TK gene (Fig. 2C, lane 4, and data not shown). A YAC with the TK and LYS2 genes inserted into its vector arm (Trp + Ura - Lys + ) was then used for the second step of recombination. Cells containing this YAC were
56 Insert
LeftArm TRP
YAC
Ri@l
I.1
Arm
Phenolype
URA3
Trp? Ura+, Lys-
-m
Trp: Ura-, Lys+ !
i TK, LYSZ -
B
I
2
3
C
4
kb
kb
350-
350-
250-
250-
150-
150-
50-
50-
I
2
Fig. 2. Adapting
YACs to promote
homologous
restriction
sites are shown.
Panels B and C: Southern in agarose
blocks
(lanes l-3)
or retrofitted
and a TK probe
recombination.
blot and hybridization
was analysed
(A) Strategy.
Recombination
vector pRV2, used in step 2 for introducing
Steps one and two are described by CHEF
analysis
gel electrophoresis
only in the YAC vector
4
TK
Nm Ehceiri et al. (1991). The recombination
3
Trpt Ura*, Lys+
marker
vector
TKLU2,
used for step 1, has been described
into insert DNA of the YAC, is diagrammed.
by
Only unique
in section b2. of DNA from yeast cells containing as described
in Fig. 1B. Results
retrofitted are shown
YACs. DNA from yeast cells immobilized for a YAC retrofitted
arms (step 1 in panel A; lanes 4). The filter was successively
hybridized
using steps
1 and 2
with a NmR probe (panel B)
(panel C).
transformed with the 5.3-kb EcoRI-BumHI fragment of plasmid pRV2. This fragment contains about 207 bp of conserved sequence of the repetitive I.1 at one end and about 306 bp at the other. Recombination of the transformed fragment in yeast should then integrate theNmR and URA3 genes by disruption of a resident Ll in the human DNA insert of the YAC. To test this expectation, Ura+ transformants were analyzed. Of 89 tested, 82 were also Trp + and Lys + , as expected. (The Lys - colonies probably arose by homologous recombination of the fragment into the YAC arm. This would replace the split URA gene (and its interstitial LYS2 gene) with an intact URA gene.) NmR insertion in the human DNA and TX: insertion in the arm of the YAC were then verified. The Trp + Ura + Lys + transformants were grown in medium lacking lysine and trypto-
phan and embedded in agarose blocks. A typical CHEF gel analysis of DNA from several colonies is presented in Fig. 2B. Hybridization with the NmR gene probe detected a YAC of the expected size (lanes 1 and 3). The filter was washed to remove the probe and was then hybridized with the TK probe to confirm the presence of the TK gene in the YAC as well (Fig. 2C). All ofthe lanes show YACs with the TK gene. One YAC gave a signal with the TK probe but not with the NmR gene probe (compare Figs. 2B and C, lane 2). It may have resulted from recombination between the split URA gene of the YAC arm and the intact URA3 gene of the vector insert, but this has not been analyzed further. Finally, to examine the number of insertions in the YAC, DNA from YACs modified to contain both TIC and NmR
57
TRP
YAC
Right Arm
Insert
Lett Arm
URA3
Ll -. )
TRP
Retrofitted YAC
NrnR. URA3
TK. LYS2
NmR, URA3
4
+
c
2
3
4
kb
kb -
I
23. I
”
ba,a-
23.1-
9.4-
6.5
6.5-
4.3-
TK
Nm Fig. 3. Presence
ofNmK and TK gene in a YAC retrofitted
retrofitted
YAC containing
fragments
generated
in both human DNA insert and vector arm. Upper panel: Schematic
a TK, LYSZ and two Nm, UL43 insertions.
by digestion
of Hind111 restriction
sites flanked
an Ll site. Lower panel: Hind111 digests of the YAC with insertion in the arm only (lane 3) and of the parental Fig. 1B. Southern to remove
transfer
the NmR probe
to duplicate
Arrows
and was then hybridized
indicate
both in the human
and subsequent
with the pBR322
putative
by LI; a’ indicates
YAC (lane 4) were fractionated
nylon membranes
PBR
probe present
genes was digested with Hind111 and analysed by conventional agarose gel electrophoresis followed by Southern blot analysis. The DNA was transferred from the gel to duplicate nylon membranes. The filters were separately probed with NmR or TK DNA. Fig. 3 (top) diagrams the expected digestion products of a YAC and a putative doubly modified YAC. Because there is no Hind111 restriction site in the DNA bearing the NmR and TK genes, DNA containing Nm R or TK is released in a fragment bounded by the nearest Hind111 sites. Thus, when treated with HindIII, the YACs shown in Fig. 2 (lanes 1 and 3) released one (Fig. 3A, lane 2) or two (Fig. 3A, lane 1) fragments containing the inserted genes. This suggests that the clones have respectively incorporated one and two copies of the NmR DNA. The presence of the TK gene in the right arm
the faster-moving
fragment
released
the corresponding
from a single insertion
at
DNA and in the vector arm (lanes 1 and 2), of a YAC retrofitted
by conventional
hybridization
of the YAC and of doubly
Hind111 sites. a, b, c, and d indicate
0.6% agarose
CHEF
gel electrophoresis
with Nm (A), and TK (B) gene probes.
as described
in
Filter A was then washed
in the right arm of the YAC (C).
of the YAC was reconfirmed by the finding of the expected fragment of similar size, corresponding to the right arm of the YAC, detected by both the TK and pBR DNA probes (Figs. 3B and C, lanes 1 and 2 compared with lane 3). The control parental YAC released a somewhat faster moving fragment ‘d’, as detected by a pBR probe (1691-bp BamHIPvuII fragment of pBR322) specific for the right vector arm (Fig. 3C, lane 4, and schematic at the top of Fig. 3). These vectors are in current use in a number of laboratories. For example, in one adaptation, YACs from human X chromosome 1~36 were modified with pRV1 and introduced into human melanoma and neuroblastoma cells. Stable NmR transformants were then selected to test for putative tumor suppressor genes in the region (T.S. Upper and S. Sarkar, personal communication).
58 (3) Applications The ease and simplicity of the manipulations in these examples and the generality of the G418/Nm selection make these vectors potentially useful for a variety of transfection studies. Other markers, targeted sites, and ways to transfer genes into mammalian cells are also coming into use. Some groups have used electroporation
of cells to introduce
DNA
(Doetschman et al., 1988) or have selected for activity of hypoxanthine-gu~ine phosphoribosyl transferase (HPRT; Szybalska and xanthine-guanine
Szybalski, 1962; Huxley et al., 1991), phosphoribosyl transferase (gpt; Jasin
and Berg, 1988), or NmR (Dorin et al., 1989) genes to promote the homologous recombination of a transfected gene at a homologous site. These techniques may also be adaptable to the retrofitting ofYACs. Also, in recent experiments, the NmR marker has been used to select for mouse embryonal carcinoma (Pavan et al., 1990) or L cells (Pachnis et al., 1990) that had incorporated a YAC by spheroplast fusion. Pavan et al. { 1990) used a vector analogous to pRV2, but which inserts the selectable marker into DNA at an Ah rather than an LI element. Ah sequences are much more frequent, and therefore provide many more potential insertion sites, although unlike the LI loci used here, the sites may not be equally homologous with the vector fragment. The selection system reported here is analogous to that of Capecchi (1989), in that both select for a clone insert and against the vector arm, enriching the transformants for homologous recombinants. However, in the earlier work, lambda recombinants that contained only portions of genes were used, and the experimental design aimed at the inactivation of a chromosomal gene. Instead, a YAC modified by pRV1 and pRV2 would likely contain even a large gene intact and in normal context, with the NmR marker in an Ll element in a non-translated region. Thus, selection for
REFERENCES Abidi, F.E., Wada,
M., Little, R.D. and Schlessinger,
chromosomes tion and
containing
human Xq24-Xq28
representation
of probe
D.: Yeast artificial
DNA: library construc-
sequences.
Cenomics
7 (1990)
363-376. Botstein,
D., Falco,
Stinchcomb, (SHY):
SC.,
Stewart,
D.T., Struhl,
a eukaryotic
Burke,
D.T., Carle,
tors
for recombi-
Isolation
of single-copy
chromosome
clones.
M.: Cloning
of large segments
of artificial
chromosome
of vec-
236 (1987) 806-812. the genome
by homologous
recombination.
244 (1989) 1288-1292.
G.F. and Olson,
Proc. Natl. Acad. T.M.,
deficiency growth
M.V.:
of yeast artificial
G.F. and Olson,
M.R.: Altering
DeChiara,
Olson,
DNA into yeast by means
Science
Science Carle,
containment
244 (1989) 1348-1351.
exogenous Capecchi,
S.,
Little, R.D., Burke, D.T., Korsmeyer,
D, and
genes from a library
Science
M., Scherer,
R.W.: Sterile host yeasts
Gene 8 (1979) 17-24.
B.H., Silverman,G.A.,
S.J., Schlessinger, human
Brennan,
system of biological
nant DNA experiments. Brownstein,
SE.,
K. and Davis,
M.V.: An electrophoretic
Efstratiadis,
phenotype
factor
karyotype
for yeast.
Sci. USA 82 (1985) 3756-3760. A. and
Robertson,
in heterozygous
II gene disrupted
E.J.:
mice carrying
by targeting.
A growth-
an insulin-like
Nature
345 (1990)
78-80. Deininger,
P.L.: SINES:
short
interspersed
repeated
higher eukaryotes.
In: Berg, D.E. and Howe,
DNA.
Society
American
pp. 61Y-637. Doetschman, T., Maeda,
for
Microbiology,
N. and Smithies,
Hprt gene in mouse embryonic
DNA element
in
M.M., (Eds.), Mobile Washington,
0.: Targeted
1989,
mutation
of the
stem cells, Proc. Natl. Acad. Sci. USA
85 (1988) 8583-8587. Dorm, J.R., Inglis, J.D. and Porteous, somal targeting Science D’Urso,
of a dominant
D.J.: Selection
for precise chromo-
marker by homologous
recombination.
243 (1989) 1357-1360.
M., Zucchi,
I., Ciccodicola,
A., Palmieri,
G., Abidi, F.E. and
Schlessinger, D.: Human glucose-6-phosphate dehydrogenase gene carried on a yeast artificial chromosome encodes active enzyme in monkey
cells. Genomics
Eibel, H. and Philippsen,
7 (1990) 531-534. P.: Identification
LYS2 gene by an integrative Genet.
of the cloned
transformation
approach.
S. cerevisiae Mol. Gen.
191 (1983) 66-73.
NmR would favor replacement of part or all of a gene rather than inactivation, with the cloned gene tending to retain its function. Such a YAC could be used for corrective repair of a defective gene by a normal copy (as discussed in Schlessinger, 1990). It remains to be seen if mutant allele replacement might also be favored by the large size of the homologous region in a YAC, in line with a trend previously noted with lambda clones (Capecchi, 1989).
Feinberg,
ACKNOWLEDGMENTS
1990, p. 9. Hutchison, C.A. III, Hardies, S.C., Loeb, D.D., Shehee, W.R. and Edgell, M.H.: LINES and related retroposons: long interspersed repeated
The work was supported by NSF grant 8406949 to D.S. and by the WU-Monsanto Research Agreement.
PMS PCM Biomedical
Eliceiri, B., Labella,
T., Hagino,
Pilia, G., Palmieri,
Y., Srivastava,
sion in mouse cells of yeast artificial genes, Proc. Natl. Acad. endonuclease
chromosomes
B.: A technique fragments
Biochem. 132 (1983) 6-13. Gnirke, A., Barnes, T., Gardiner, M.V.: Cloning and expression
sequences
in the eukaryotic
Mobile
DNA.
ington,
1989, pp. 593-619.
harboring
for radiolabeling
to higher specific activity.
K., Patterson, of the human
artificial chromosomes. Genome Mapping Abstract. Cold Spring Harbor Laboratory,
(Eds.),
D.,
and expreshuman
Sci. USA 88 (1991) 2179-2183.
A, and Vogelstein,
restriction
A.K., Schlessinger,
G. and D’Urso, M.: Stable integration
DNA Anal.
D., Schild, D. and Olson, GART locus using yeast and Sequencing Meeting Cold Spring Harbor, NY,
genome. In: Berg, DE. and Howe, M.M.,
American
Society
for Microbiology,
Wash-
59 Huxley,
C., Hagino,
HPRT
transferred Jasin,
Y., Schlessinger,
gene on a yeast
D. and Olson,
artificial
chromosome
to mouse cells by cell fusion. Genomics
M. and Berg, P.: Homologous
without Labella,
target
gene selection.
T. and Schlessinger,
integration
Genes
that expresses
rDNA
Genomics
cells units
5 (1989) 752-760.
J. and Varmus,
tumor
virus
regulation
Laboratory
Scott,A.F.,
Harbor,
trait. Mol. Cell.
repeat
of the mouse
confers
mammary
glucocorticoid
Singer,
hormone
S.L., Thomas,
proto-oncogene strategy
gene. Proc. Natl. Acad. Sci. USA
Sambrook,
Cold Spring
Harbor
J.: Molecular Laboratory,
Cloning.
A
Cold Spring
M.R.: Disruption
of the
stem cells: a general
to non-selectable
genes. Nature
336
(1988) 348-352. Pachnis,
artificial
P., Rothstein, chromosome
R. and Costantini, carrying
myces cerevisiae into mammalian
human
DNA
F.: Transfer
of a
from Saccharo-
cells. Proc. Nat]. Acad. Sci. USA 87
(1990) 5109-5113. Pavan,
carcinoma
yeast artificial
chromosome.
cell line of a 360-kilobase
and transfer
into
human-derived
Mol. Cell. Biol. 10 (1990) 4163-4169.
Sci. USA 87
M., Comey, C.T., O’Hara,
B.,
P., Smith, K.D. and Margolet,
L.:
proposed
DNA sequence.
repeat
progenitor
Genomics
J.: Making
sequence
and
6 (1990) 248-258.
in
genes deduced
1 (1987) 113-125.
sense out of LINES:
mammalian
genome.
long Trends
Sci. 10 (1985) 119-122.
DNA-mediated Natl. Acad.
heritable
W.: Genetics
transformation
of human
cell lines, IV.
of a biochemical
trait. Proc.
Sci. USA 48 (1962) 2026-2034.
K.R. and Capecchi,
targeting
in mouse
M.R.: Site-directed
embryo-derived
mutagenesis
stem cells. Nature
by gene 346 (1990)
847-850. Traver,
C.N.,
Klapholz,
S., Hyman,
R.W.
and
Davis,
R.W.:
Rapid
of a human genomic library in yeast artificial chromosomes
for single copy sequences.
Proc.
Natl. Acad.
Sci. USA
86 (1989)
5898-5902. Yanisch-Perron, cloning
W.J., Hieter, P. and Reeves, R.H.: Modification
an embryonal
elefor its
tools for mapping
Genetics
B.J., Abdelrazik,
E.H. and Szybalski,
screening
V., Larysa,
yeast
Biochem.
Thomas, K.R. and Cappecchi, mutations
Trends
J.P., Cooley, T., Heath,
M.F. and Skowronski,
Szybalska,
int-2 in mouse embryo-derived
for targeting
chromosomes:
genomes.
Schmeckeper,
interspersed
NY, 1982.
Mansour,
of complex
from a consensus
E.F. and
Manual.
D.: Yeast artificial
analysis
Origin ofthe human LZ elements:
selective
B.H.: Regulatory
gene are necessary
stem cells. Proc. Natl. Acad.
a dominant
on a linked heterologous
T., Fritsch,
in embryonic
HPRT
(1990) 4299-4303.
Rossiter,
H.E.: A small region
long terminal
0. and Keller,
of the human
P.M.: A stable bovine papillomavirus
80 (1983) 5866-5870. Maniatis,
R.G., Smithies,
ments in the introns
Schlessinger,
repeat
Biol. 3 (1983) 2110-2115. Majors,
Reid, L.H., Gregg, expression
9 (1991) 742-750.
in mammalian
human
isolated in yeast artificial chromosomes. plasmid
when
Dev. 2 (1988) 1353-1366.
D.: Complete
Law, M., Byrne, J.C. and Howley, hybrid
M.: The human
is functional
M13mp18
C., Vieira,
vectors
and
and pUC19
J. and Messing, host
strains:
vectors.
J.: Improved
nucleotide
Ml3
sequences
Gene 33 (1985) 103-119.
phage of the
GENE
Publishers
B.V. All rights reserved.
53
0378-l 119/91/$03.50
05026
Vectors for inserting selectable markers in vector arms and human DNA inserts of yeast artificial chromosomes (YACs) (Homologous
recombination;
plasmid;
neomycin
resistance;
LYS2 gene; LI element;
thymidine
kinase;
recombinant
DNA)
Anand K. Srivastava and David Schlessinger Department of Molecular Microbiology and Center for Genetics in Medicine, Washington UniversitySchool of Medicine, St. Louis, MO 63110 (U.S.A.) Received by G.N. Gussin: 17 December Revised: 8 March 1991 Accepted: 13 March 1991
1990
SUMMARY
To facilitate studies of gene expression and homologous recombination, plasmids have been developed which permit the insertion of neomycin resistance-encoding gene (NmR) into either the human DNA insert or the vector arm of a yeast artificial chromosome (YAC). To integrate into the YAC arm, the plasmid pRV1 contains a LYS2 (encoding a-aminoadipate reductase) gene for selection in the yeast host, and a NmR gene for subsequent selection after transfection of mammalian cells. These two sequences are bracketed by fragments of the URA3 gene (encoding orotidine-5’-phosphate decarboxylase) that can disrupt the URA3 gene in the YAC arm by homologous recombination in yeast. To integrate a selectable marker into the insert, the plasmid pRV2 contains a NmR gene and an intact copy of the URA3 gene, bracketed by segments of an LI (LINES) repetitive element. In this case, the vector has been designed for use with YACs that have already been fitted in the vector arm with a different marker (i.e., TK) that has disrupted the URA3 gene in the vector arm. Selection is for the restoration of URA3 gene activity attendant on recombination into an Ll element in the YAC insert. Use of the vectors is illustrated with a YAC clone containing ribosomal DNA.
Transfection studies of DNA constructs have become a standard way to examine the function of gene sequences. The size of DNA fragments that can be accommodated in traditional bacterial and phage vectors has been limited, however. Consequently, for many genes, it was difficult to
achieve constructs with the signals required for a number of regulatory phenomena, including tissue-specific expression and mRNA metabolism (DeChiara et al., 1990; Reid et al., 1990). The introduction of vectors in which large DNA inserts can be maintained has provided potential reagents for the study of even large genes. The YACs (Burke et al., 1987)
Correspondence to: Dr. D. Schlessinger, Department of Molecular Microbiology, Washington University School of Medicine, St. Louis, MO
LYS2, gene encoding
63110 (U.S.A.)
gene encoding
INTRODUCTION
Tel. (314)362-2744;
Fax (314)362-1232.
cation; encoding
Abbreviations: aa, amino acid(s); Ap, ampicillin; bp, base pair(s); CHEF, contour-clamped hexagonal electrophoresis; EtdBr, ethidium bromide;
Ll (LINES), large interspersed
kb, kilobase(
a-aminoadipate
Nm resistance;
PFGE,
pulsed-field
nt, nucleotide(s); gel electrophoresis;
TK; TK, thymidine
ribosylanthranilate phate decarboxylase;
reductase;
isomerase;
kinase;
repeated
sequence(s);
Nm, neomycin; r, ribosomal;
TRPI, gene encoding
URA3, gene encoding
YAC, yeast artificial
NmR,
on’, origin of DNA repliTK, gene phospho-
orotidine-5’-phos-
chromosome.
54 in particular, can be used to clone most genes in complete form and in normal sequence context. For example, YAC cloning has permitted the recovery of intact genes, including factor VIII (Abidi et al., 1990) factor IX (Brownstein et al., 1989) glucose-6-phosphate dehydrogenase (G6PD gene; D’Urso et al., 1990) and glycineamide ribonucleotide transformylase (GART gene; Gnirke et al., 1990); the last two have been shown to produce active enzyme from YACs upon transfection of mammalian cells (D’Urso et al., 1990; Gnirke et al., 1990). To investigate the expression and fate of YACs in detail, it is necessary to establish them stably in recipient cells. A selective marker can be part of the YAC vector when a library is constructed (Traver et al., 1989); but a large number of currently available YACs contain no such marker including the original and still widely used pYAC4 (Burke et al., 1987). For those, modification of the existing YAC with appropriate markers, a process that has been called ‘retrofitting’, is indispensible. We have reported one vector (TKLU2) which can be used to introduce the selectable TK gene into the vector arm of a YAC (Eliceiri et al., 1991). This facilitates the subsequent selection of TK-deficient mammalian cells that have been stably transformed with the modified YAC (Eliceiri et al., 1991). Use of the TK gene as a selective marker is restricted to cell lines deficient for the gene. Here we describe two additional vectors, pRV1 and pRV2, which extend the use of such a system to mammalian cells in general. Both plasmids contain the NmR gene, a marker selectable in mammalian cells, and can introduce it, respectively, into a dispensible portion of a YAC (the vector arm) or into the insert DNA of a YAC. Adding Nm R to the vector arm with pRV 1 permits direct transfection studies. With a similar aim, NmR has been introduced into a repetitive sequence (Ah) in the human insert of a YAC (Pavan et al., 1990). In contrast, rather than fitting a YAC directly with the NmR gene in the insert, pRV2 is designed to be used in a second step with YACs that have already been retrofitted with the TK gene in the vector arm. As a result of the successive use of the two vectors TKLU2 and pRV2, YACs are recovered that permit one to select for the NmR marker in the insert and against the TK marker in the arm. This imitates in YACs the positive-negative selection system developed by Mansour et al. (1988) (see Thomas and Capecchi, 1990) to promote gene alteration by a homologous copy in a 2 phage.
obviate the need to make YACs with vectors that commit one to the use of only a particular selective marker, and free one from the dependence on available restriction sites for recombinant DNA manipulations. (a) Retrofitting YAC vectors arms with the NmR gene In construct pRV1 (Fig. 1) the NmR and LYS2 genes were inserted at a unique site within the URA3 gene. Construction was begun by subcloning a 3.7-kb EcoRI-BamHI fragment of plasmid pdBPV-MMTneo (Law et al., 1983) containing the NmR gene, between the EcoRI and BamHI sites of pUC18 (Yanisch-Perron et al., 1985). The resulting plasmid, pNm, was linearized with BamHI. The ends were made flush using the Klenow fragment of E. co/i DNA polymerase I and dNTPs, and the terminal phosphates were then removed by calf thymus alkaline phosphatase (Maniatis et al., 1982). A 5.2-kb EcoRI-Hind111 fragment of plasmid YIp333 (Eibel and Philippsen, 1983) containing the LYS2 gene, which had also been rendered blunt-ended
A
B kb 450350 -
I
Nlll
Fig. 1. Targeting ofthe Nmamarker into a YAC vector arm. (A) Diagram of retrofitting vector pRV1. Only unique restriction sites are shown. (B) PFGE
analysis
were grown
lysine
described
of seven clones (Trp + Ura-
in synthetic
liquid medium
and tryptophan,
low-melting-agarose AND DISCUSSION
blocks
gel shows
and
Lys2 + ). Transformants
supplemented
DNA
yeast
DNA transferred
with aa mixture
was immobilized
and fractionated
in a CHEF
by Carle and Olson (1985). A 1% agarose
TBE buffer with switching
The highly recombinogenic nature of yeast facilitates the modification of resident YACs to incorporate markers that can promote their retention in mammalian cells by selection. Standard techniques of gene disruption and insertion
3456769
7
lacking RESULTS
2 1 .
in 0.5”;
apparatus
as
gel was run in 0.5X
time of 15 s to 30 s for 20 h. The EtdBr-stained
chromosomes
and YACs.
to a nylon membrane
(C)Autoradiogram
(Sureblot,
Oncor)
of the
from the gel
in panel B and hybridized to NmR probe DNA. Lanes 1-3 and 5-8, YACs; lane 9, parental YAC; lane 4, marker of concatamerized I genomes. Arrow
indicates
the position
of YACs.
55 as above, was then ligated to the linear blunt-ended plasmid. The EcoRI-Hind111
fragment
of the plasmid
pNm
bearing the
fused NmR and LYS2 genes was made blunt-ended as described above, repurified, and inserted at a unique Stul site within the URA3 gene [contained on the Hind111 restriction fragment of plasmid YEP24; Botstein et al. (1978) and cloned into the Hind111 site of pUCl8 (Yanisch-Perron et al., 1985)]. Digestion of plasmid pRV1 with Hind111 (Fig. 1A) released a 9.5-kb fragment containing the LYS2 and Nm R genes between segments of the yeast URA3 gene.
513-bp
HinfI-SnaBI
fragment
portion
of a human
Ll
repeat
containing
a 3’-conserved
was isolated
from pCD
KpnI-8 (Scott et al., 1987) and cloned into the SmaI site of pUCl8.) Since LI elements are not present in yeast DNA, LI in the vector should selectively recombine into the Ll of the human DNA insert of YACs. LI have several advantages as a target for the introduction of selectable markers in the human DNA inserts of YACs. These include: (i) Their frequency. LI occurs about once every 50 kb in total human DNA (Singer and Skowronski, 1985) and would therefore likely occur several times in typical YACs
Integrative disruption of the URA3 gene in the YAC arm by this fragment produced recombinants that had become
of 100 to 600 kb. Thus, the selective marker can be intro-
Lys’ Ura in yeast and contained the Nm R gene. In pilot experiments, pRV1 was used to introduce
duced at a fixed number of sites, making it flexible enough to yield a probable insertion at a site useful for a variety of
the
NmR marker into several YAC clones. For example, yeast carrying yA16G4, a YAC clone containing human rDNA (Labella and Schlessinger, 1989) was transformed with 0.25, 0.5 and 1.0 pg of gel-purified pRV1 fragment by the spheroplasting procedure (Burke et al., 1987). From several experiments, 96 colonies were selected for growth in the absence of lysine (due to the L YS2 gene in the right arm of the YAC) and tryptophan (due to the TRPI gene in the left arm of the YAC). Of the 96, 69 were also Ura- (the other strains may have undergone recombination into the already inactive chromosomal URA3 gene, and thus retained an intact homologue in the YAC arm). DNA from seven randomly chosen transformants was fractionated by PFGE (Carle and Olson, 1985) (Fig. 1B). The normal distribution of yeast chromosomes in the range of 200 to 500 kb is seen in the EtdBr-stained gel, along with the modified YACs. Five of the seven contained a 160-kb YAC, as expected (lanes 3 and 5-8); lane 9 shows the smaller parental YAC before modification. The DNA was transferred to a nylon membrane and analyzed by hybridization with probes that included a 3.7-kb EcoRI-BamHI fragment of pdBPVMMTneo containing the NmR gene (Law et al., 1985) and labeled using the random primer method of Feinberg and Vogelstein (1983). Fig. 1C indicates that the five YACs of the anticipated size also contained NmR gene sequences. Insertion of the NmR gene into the YAC was also verified by analysis of the products of restriction enzyme digestion (data not shown). (b) Adapting YACs to promote homologous in human cells
recombination
(1) Principles of using Ll element To introduce the mammalian selectable marker (NmR) into the human DNA insert of a YAC, we capitalized on the occurrence of repetitive LINES (LZ) elements (Scott et al., 1987) in human DNA. Vector pRV2 contains a NmR cassette and a URA3 gene between human LI repeats. (A
purposes, but infrequent enough to be relatively easy to map the site of insertion in the YAC. (ii) Their constancy. The part of Ll outside the portion used varies almost as much as Ah sequences (Deininger, 1989) and can be ofhighly variable length (Hutchison et al., 1989); but the segment employed (517 nt at the 3’ end) is highly conserved in the range of Ll in the human genome. This makes it highly likely that the transforming fragment will be inserted at a comparable site in the repetitive sequence in all cases, and with a comparable chance of recombining with every Ll element. (2) Procedures The vector pRV2 is designed to be used in a two-step procedure (Fig. 2A) to put a positive selectable marker into the insert of a YAC and a negative selectable marker into the vector arm. In step one, using vector TKLU2 (Eliceiri et al., 1991), a YAC was first modified by insertion of the TK gene into the URA3 gene in the YAC vector arm. Yeast cells carrying a YAC with the resultant Trp + Ura- Lys + phenotype were selected and the NmR gene was inserted into their human DNA moiety using the vector pRV2. The final recombinants were Trp’ Lys’ and had the Ura+ phenotype restored (Fig. 2A). This strategy was tested on the same YAC (yAl6G4) used in Fig. 1. The presence of LI in this YAC had already been confirmed, making it feasible to insert DNA at those sites. Yeast cells containing the YAC were transformed with the Hind111 restriction fragment of plasmid TKLU2 containing the TK and LYS2 genes. Insertion of the TK gene into the vector arm of several of the Trp + Ura- Lys + YACs was verified by restriction analysis, and by hybridization with a probe that included a 2040-bp PvuII fragment of plasmid TK321 (Majors and Varmus, 1983) containing the TK gene (Fig. 2C, lane 4, and data not shown). A YAC with the TK and LYS2 genes inserted into its vector arm (Trp + Ura - Lys + ) was then used for the second step of recombination. Cells containing this YAC were
56 Insert
LeftArm TRP
YAC
Ri@l
I.1
Arm
Phenolype
URA3
Trp? Ura+, Lys-
-m
Trp: Ura-, Lys+ !
i TK, LYSZ -
B
I
2
3
C
4
kb
kb
350-
350-
250-
250-
150-
150-
50-
50-
I
2
Fig. 2. Adapting
YACs to promote
homologous
restriction
sites are shown.
Panels B and C: Southern in agarose
blocks
(lanes l-3)
or retrofitted
and a TK probe
recombination.
blot and hybridization
was analysed
(A) Strategy.
Recombination
vector pRV2, used in step 2 for introducing
Steps one and two are described by CHEF
analysis
gel electrophoresis
only in the YAC vector
4
TK
Nm Ehceiri et al. (1991). The recombination
3
Trpt Ura*, Lys+
marker
vector
TKLU2,
used for step 1, has been described
into insert DNA of the YAC, is diagrammed.
by
Only unique
in section b2. of DNA from yeast cells containing as described
in Fig. 1B. Results
retrofitted are shown
YACs. DNA from yeast cells immobilized for a YAC retrofitted
arms (step 1 in panel A; lanes 4). The filter was successively
hybridized
using steps
1 and 2
with a NmR probe (panel B)
(panel C).
transformed with the 5.3-kb EcoRI-BumHI fragment of plasmid pRV2. This fragment contains about 207 bp of conserved sequence of the repetitive I.1 at one end and about 306 bp at the other. Recombination of the transformed fragment in yeast should then integrate theNmR and URA3 genes by disruption of a resident Ll in the human DNA insert of the YAC. To test this expectation, Ura+ transformants were analyzed. Of 89 tested, 82 were also Trp + and Lys + , as expected. (The Lys - colonies probably arose by homologous recombination of the fragment into the YAC arm. This would replace the split URA gene (and its interstitial LYS2 gene) with an intact URA gene.) NmR insertion in the human DNA and TX: insertion in the arm of the YAC were then verified. The Trp + Ura + Lys + transformants were grown in medium lacking lysine and trypto-
phan and embedded in agarose blocks. A typical CHEF gel analysis of DNA from several colonies is presented in Fig. 2B. Hybridization with the NmR gene probe detected a YAC of the expected size (lanes 1 and 3). The filter was washed to remove the probe and was then hybridized with the TK probe to confirm the presence of the TK gene in the YAC as well (Fig. 2C). All ofthe lanes show YACs with the TK gene. One YAC gave a signal with the TK probe but not with the NmR gene probe (compare Figs. 2B and C, lane 2). It may have resulted from recombination between the split URA gene of the YAC arm and the intact URA3 gene of the vector insert, but this has not been analyzed further. Finally, to examine the number of insertions in the YAC, DNA from YACs modified to contain both TIC and NmR
57
TRP
YAC
Right Arm
Insert
Lett Arm
URA3
Ll -. )
TRP
Retrofitted YAC
NrnR. URA3
TK. LYS2
NmR, URA3
4
+
c
2
3
4
kb
kb -
I
23. I
”
ba,a-
23.1-
9.4-
6.5
6.5-
4.3-
TK
Nm Fig. 3. Presence
ofNmK and TK gene in a YAC retrofitted
retrofitted
YAC containing
fragments
generated
in both human DNA insert and vector arm. Upper panel: Schematic
a TK, LYSZ and two Nm, UL43 insertions.
by digestion
of Hind111 restriction
sites flanked
an Ll site. Lower panel: Hind111 digests of the YAC with insertion in the arm only (lane 3) and of the parental Fig. 1B. Southern to remove
transfer
the NmR probe
to duplicate
Arrows
and was then hybridized
indicate
both in the human
and subsequent
with the pBR322
putative
by LI; a’ indicates
YAC (lane 4) were fractionated
nylon membranes
PBR
probe present
genes was digested with Hind111 and analysed by conventional agarose gel electrophoresis followed by Southern blot analysis. The DNA was transferred from the gel to duplicate nylon membranes. The filters were separately probed with NmR or TK DNA. Fig. 3 (top) diagrams the expected digestion products of a YAC and a putative doubly modified YAC. Because there is no Hind111 restriction site in the DNA bearing the NmR and TK genes, DNA containing Nm R or TK is released in a fragment bounded by the nearest Hind111 sites. Thus, when treated with HindIII, the YACs shown in Fig. 2 (lanes 1 and 3) released one (Fig. 3A, lane 2) or two (Fig. 3A, lane 1) fragments containing the inserted genes. This suggests that the clones have respectively incorporated one and two copies of the NmR DNA. The presence of the TK gene in the right arm
the faster-moving
fragment
released
the corresponding
from a single insertion
at
DNA and in the vector arm (lanes 1 and 2), of a YAC retrofitted
by conventional
hybridization
of the YAC and of doubly
Hind111 sites. a, b, c, and d indicate
0.6% agarose
CHEF
gel electrophoresis
with Nm (A), and TK (B) gene probes.
as described
in
Filter A was then washed
in the right arm of the YAC (C).
of the YAC was reconfirmed by the finding of the expected fragment of similar size, corresponding to the right arm of the YAC, detected by both the TK and pBR DNA probes (Figs. 3B and C, lanes 1 and 2 compared with lane 3). The control parental YAC released a somewhat faster moving fragment ‘d’, as detected by a pBR probe (1691-bp BamHIPvuII fragment of pBR322) specific for the right vector arm (Fig. 3C, lane 4, and schematic at the top of Fig. 3). These vectors are in current use in a number of laboratories. For example, in one adaptation, YACs from human X chromosome 1~36 were modified with pRV1 and introduced into human melanoma and neuroblastoma cells. Stable NmR transformants were then selected to test for putative tumor suppressor genes in the region (T.S. Upper and S. Sarkar, personal communication).
58 (3) Applications The ease and simplicity of the manipulations in these examples and the generality of the G418/Nm selection make these vectors potentially useful for a variety of transfection studies. Other markers, targeted sites, and ways to transfer genes into mammalian cells are also coming into use. Some groups have used electroporation
of cells to introduce
DNA
(Doetschman et al., 1988) or have selected for activity of hypoxanthine-gu~ine phosphoribosyl transferase (HPRT; Szybalska and xanthine-guanine
Szybalski, 1962; Huxley et al., 1991), phosphoribosyl transferase (gpt; Jasin
and Berg, 1988), or NmR (Dorin et al., 1989) genes to promote the homologous recombination of a transfected gene at a homologous site. These techniques may also be adaptable to the retrofitting ofYACs. Also, in recent experiments, the NmR marker has been used to select for mouse embryonal carcinoma (Pavan et al., 1990) or L cells (Pachnis et al., 1990) that had incorporated a YAC by spheroplast fusion. Pavan et al. { 1990) used a vector analogous to pRV2, but which inserts the selectable marker into DNA at an Ah rather than an LI element. Ah sequences are much more frequent, and therefore provide many more potential insertion sites, although unlike the LI loci used here, the sites may not be equally homologous with the vector fragment. The selection system reported here is analogous to that of Capecchi (1989), in that both select for a clone insert and against the vector arm, enriching the transformants for homologous recombinants. However, in the earlier work, lambda recombinants that contained only portions of genes were used, and the experimental design aimed at the inactivation of a chromosomal gene. Instead, a YAC modified by pRV1 and pRV2 would likely contain even a large gene intact and in normal context, with the NmR marker in an Ll element in a non-translated region. Thus, selection for
REFERENCES Abidi, F.E., Wada,
M., Little, R.D. and Schlessinger,
chromosomes tion and
containing
human Xq24-Xq28
representation
of probe
D.: Yeast artificial
DNA: library construc-
sequences.
Cenomics
7 (1990)
363-376. Botstein,
D., Falco,
Stinchcomb, (SHY):
SC.,
Stewart,
D.T., Struhl,
a eukaryotic
Burke,
D.T., Carle,
tors
for recombi-
Isolation
of single-copy
chromosome
clones.
M.: Cloning
of large segments
of artificial
chromosome
of vec-
236 (1987) 806-812. the genome
by homologous
recombination.
244 (1989) 1288-1292.
G.F. and Olson,
Proc. Natl. Acad. T.M.,
deficiency growth
M.V.:
of yeast artificial
G.F. and Olson,
M.R.: Altering
DeChiara,
Olson,
DNA into yeast by means
Science
Science Carle,
containment
244 (1989) 1348-1351.
exogenous Capecchi,
S.,
Little, R.D., Burke, D.T., Korsmeyer,
D, and
genes from a library
Science
M., Scherer,
R.W.: Sterile host yeasts
Gene 8 (1979) 17-24.
B.H., Silverman,G.A.,
S.J., Schlessinger, human
Brennan,
system of biological
nant DNA experiments. Brownstein,
SE.,
K. and Davis,
M.V.: An electrophoretic
Efstratiadis,
phenotype
factor
karyotype
for yeast.
Sci. USA 82 (1985) 3756-3760. A. and
Robertson,
in heterozygous
II gene disrupted
E.J.:
mice carrying
by targeting.
A growth-
an insulin-like
Nature
345 (1990)
78-80. Deininger,
P.L.: SINES:
short
interspersed
repeated
higher eukaryotes.
In: Berg, D.E. and Howe,
DNA.
Society
American
pp. 61Y-637. Doetschman, T., Maeda,
for
Microbiology,
N. and Smithies,
Hprt gene in mouse embryonic
DNA element
in
M.M., (Eds.), Mobile Washington,
0.: Targeted
1989,
mutation
of the
stem cells, Proc. Natl. Acad. Sci. USA
85 (1988) 8583-8587. Dorm, J.R., Inglis, J.D. and Porteous, somal targeting Science D’Urso,
of a dominant
D.J.: Selection
for precise chromo-
marker by homologous
recombination.
243 (1989) 1357-1360.
M., Zucchi,
I., Ciccodicola,
A., Palmieri,
G., Abidi, F.E. and
Schlessinger, D.: Human glucose-6-phosphate dehydrogenase gene carried on a yeast artificial chromosome encodes active enzyme in monkey
cells. Genomics
Eibel, H. and Philippsen,
7 (1990) 531-534. P.: Identification
LYS2 gene by an integrative Genet.
of the cloned
transformation
approach.
S. cerevisiae Mol. Gen.
191 (1983) 66-73.
NmR would favor replacement of part or all of a gene rather than inactivation, with the cloned gene tending to retain its function. Such a YAC could be used for corrective repair of a defective gene by a normal copy (as discussed in Schlessinger, 1990). It remains to be seen if mutant allele replacement might also be favored by the large size of the homologous region in a YAC, in line with a trend previously noted with lambda clones (Capecchi, 1989).
Feinberg,
ACKNOWLEDGMENTS
1990, p. 9. Hutchison, C.A. III, Hardies, S.C., Loeb, D.D., Shehee, W.R. and Edgell, M.H.: LINES and related retroposons: long interspersed repeated
The work was supported by NSF grant 8406949 to D.S. and by the WU-Monsanto Research Agreement.
PMS PCM Biomedical
Eliceiri, B., Labella,
T., Hagino,
Pilia, G., Palmieri,
Y., Srivastava,
sion in mouse cells of yeast artificial genes, Proc. Natl. Acad. endonuclease
chromosomes
B.: A technique fragments
Biochem. 132 (1983) 6-13. Gnirke, A., Barnes, T., Gardiner, M.V.: Cloning and expression
sequences
in the eukaryotic
Mobile
DNA.
ington,
1989, pp. 593-619.
harboring
for radiolabeling
to higher specific activity.
K., Patterson, of the human
artificial chromosomes. Genome Mapping Abstract. Cold Spring Harbor Laboratory,
(Eds.),
D.,
and expreshuman
Sci. USA 88 (1991) 2179-2183.
A, and Vogelstein,
restriction
A.K., Schlessinger,
G. and D’Urso, M.: Stable integration
DNA Anal.
D., Schild, D. and Olson, GART locus using yeast and Sequencing Meeting Cold Spring Harbor, NY,
genome. In: Berg, DE. and Howe, M.M.,
American
Society
for Microbiology,
Wash-
59 Huxley,
C., Hagino,
HPRT
transferred Jasin,
Y., Schlessinger,
gene on a yeast
D. and Olson,
artificial
chromosome
to mouse cells by cell fusion. Genomics
M. and Berg, P.: Homologous
without Labella,
target
gene selection.
T. and Schlessinger,
integration
Genes
that expresses
rDNA
Genomics
cells units
5 (1989) 752-760.
J. and Varmus,
tumor
virus
regulation
Laboratory
Scott,A.F.,
Harbor,
trait. Mol. Cell.
repeat
of the mouse
confers
mammary
glucocorticoid
Singer,
hormone
S.L., Thomas,
proto-oncogene strategy
gene. Proc. Natl. Acad. Sci. USA
Sambrook,
Cold Spring
Harbor
J.: Molecular Laboratory,
Cloning.
A
Cold Spring
M.R.: Disruption
of the
stem cells: a general
to non-selectable
genes. Nature
336
(1988) 348-352. Pachnis,
artificial
P., Rothstein, chromosome
R. and Costantini, carrying
myces cerevisiae into mammalian
human
DNA
F.: Transfer
of a
from Saccharo-
cells. Proc. Nat]. Acad. Sci. USA 87
(1990) 5109-5113. Pavan,
carcinoma
yeast artificial
chromosome.
cell line of a 360-kilobase
and transfer
into
human-derived
Mol. Cell. Biol. 10 (1990) 4163-4169.
Sci. USA 87
M., Comey, C.T., O’Hara,
B.,
P., Smith, K.D. and Margolet,
L.:
proposed
DNA sequence.
repeat
progenitor
Genomics
J.: Making
sequence
and
6 (1990) 248-258.
in
genes deduced
1 (1987) 113-125.
sense out of LINES:
mammalian
genome.
long Trends
Sci. 10 (1985) 119-122.
DNA-mediated Natl. Acad.
heritable
W.: Genetics
transformation
of human
cell lines, IV.
of a biochemical
trait. Proc.
Sci. USA 48 (1962) 2026-2034.
K.R. and Capecchi,
targeting
in mouse
M.R.: Site-directed
embryo-derived
mutagenesis
stem cells. Nature
by gene 346 (1990)
847-850. Traver,
C.N.,
Klapholz,
S., Hyman,
R.W.
and
Davis,
R.W.:
Rapid
of a human genomic library in yeast artificial chromosomes
for single copy sequences.
Proc.
Natl. Acad.
Sci. USA
86 (1989)
5898-5902. Yanisch-Perron, cloning
W.J., Hieter, P. and Reeves, R.H.: Modification
an embryonal
elefor its
tools for mapping
Genetics
B.J., Abdelrazik,
E.H. and Szybalski,
screening
V., Larysa,
yeast
Biochem.
Thomas, K.R. and Cappecchi, mutations
Trends
J.P., Cooley, T., Heath,
M.F. and Skowronski,
Szybalska,
int-2 in mouse embryo-derived
for targeting
chromosomes:
genomes.
Schmeckeper,
interspersed
NY, 1982.
Mansour,
of complex
from a consensus
E.F. and
Manual.
D.: Yeast artificial
analysis
Origin ofthe human LZ elements:
selective
B.H.: Regulatory
gene are necessary
stem cells. Proc. Natl. Acad.
a dominant
on a linked heterologous
T., Fritsch,
in embryonic
HPRT
(1990) 4299-4303.
Rossiter,
H.E.: A small region
long terminal
0. and Keller,
of the human
P.M.: A stable bovine papillomavirus
80 (1983) 5866-5870. Maniatis,
R.G., Smithies,
ments in the introns
Schlessinger,
repeat
Biol. 3 (1983) 2110-2115. Majors,
Reid, L.H., Gregg, expression
9 (1991) 742-750.
in mammalian
human
isolated in yeast artificial chromosomes. plasmid
when
Dev. 2 (1988) 1353-1366.
D.: Complete
Law, M., Byrne, J.C. and Howley, hybrid
M.: The human
is functional
M13mp18
C., Vieira,
vectors
and
and pUC19
J. and Messing, host
strains:
vectors.
J.: Improved
nucleotide
Ml3
sequences
Gene 33 (1985) 103-119.
phage of the