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J Virol, April 1998, p. 3501-3503, Vol. 72, No. 4
Avian Disease and Oncology Laboratory,
Agricultural Research Service, USDA, East Lansing, Michigan
48823,1 and
Department of Microbiology
and Molecular Genetics, Harvard Medical School, Boston,
Massachusetts 021152
Received 5 August 1997/Accepted 6 December 1997
Host susceptibility to subgroup B, D, and E avian leukosis viruses
(ALV) is determined by specific alleles of the chicken tvb
locus. Recently, a chicken gene that encodes a cellular receptor, designated CAR1, specific for subgroups B and D ALV was cloned, and it
was proposed that this gene was the s3 allele of
tvb (J. Brojatsch, J. Naughton, M. M. Rolls, K. Zingler, and J. A. T. Young, Cell 87:845-855, 1996). We now
report that in a backcross derived from an F1 (Jungle
Fowl × White Leghorn [WL]) male mated with inbred WL females,
the cloned ALV receptor gene cosegregated with two markers linked to
tvb. The two markers used were a
tvbs1-specific antigen recognized by the
chicken R2 alloantiserum and restriction fragment length polymorphisms
associated with the expressed sequence tag com152e. With all three
markers, no crossovers were observed among 52 backcross progeny tested
and LOD linkage scores of 15.7 were obtained. These data demonstrate
that CAR1 is the subgroup B and D ALV susceptibility gene
located at tvbs3.
Based on host range and viral
interference patterns, avian leukosis viruses (ALV) isolated from
chickens are classified into six major subgroups (A to E and J). Host
susceptibility to infection by members of subgroups ALV-B, ALV-D, and
ALV-E is governed by the autosomal tvb locus, thought to
encode cellular receptors for these viruses (for a review, see
reference 12). Functionally distinct alleles of this
chicken locus have been identified: tvbs1
permits infection by these three viral subgroups;
tvbs3 permits infection only by ALV-B and ALV-D;
and the recessive tvbr allele does not permit
entry by any of these viruses (for a review, see reference
12). We recently identified CAR1, a
chicken gene that encodes a tumor necrosis factor receptor-related
protein, which is a cellular receptor specific for ALV-B and ALV-D
(3). We have also identified SEAR, a protein encoded by the
apparent turkey homolog of CAR1, which is a cellular
receptor for ALV-E (1). Based upon the properties of
CAR1, we proposed that it was the s3 allele of
tvb (3).
To determine whether CAR1 maps to tvb, we
initially attempted to identify specific restriction fragment length
polymorphisms (RFLPs) that could be used to follow the segregation of
distinct alleles of the cloned gene in a cross between chickens with
different tvb genotypes. Genomic DNA from line
63 (tvbs1 homozygotes) and from line
72 (tvbr homozygotes) (2)
was subjected to Southern blot analysis (10) with a
radioactively labeled CAR1-specific DNA fragment as a probe. With a number of enzymes tested, this probe detected a unique DNA
restriction fragment (Fig. 1), indicating
that there are no other chicken genes highly related to
CAR1. However, the CAR1 alleles from both chicken
lines were highly conserved, as judged by the similarly sized DNA
restriction fragments (Fig. 1). Indeed, when a panel of more than 50 independent restriction enzymes was used, identical patterns of DNA
restriction fragments that cross-hybridized with the probe were
detected with both types of CAR1 allele (data not shown).
Therefore, RFLP analysis proved not to be a useful method for mapping
CAR1.
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
The CAR1 Gene Encoding a Cellular Receptor Specific for
Subgroup B and D Avian Leukosis Viruses Maps to the Chicken
tvb Locus
ABSTRACT
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FIG. 1.
Southern blot analysis of CAR1 in two chicken
lines with different tvb genotypes. Samples of 5 µg of
genomic DNA from chickens of line 63 (homozygous
for tvbs1; labeled as s1) and of line
72 (homozygous for tvbr; labeled as
r) were digested with AflIII, BclI,
Bsu36I, and HincII, electrophoresed on a 1%
agarose gel, and transferred to a nylon membrane (Hybond; Amersham)
(10). The membrane was then probed at 65°C with two
radioactively labeled EcoRI restriction DNA fragments (1.5 and 1.9 kb in size) derived from a genomic clone of
CAR1 (3), by using previously described
hybridization and washing conditions (4).
Instead, a PCR-based method was used for mapping (described below) that distinguished between alleles of CAR1 from Jungle Fowl (JF) and White Leghorn (WL) chickens. JF and WL chicken lines are known to differ at tvb because the R2 alloantiserum, which recognizes a tvbs1-specific antigen, bound to cells from JF but not WL chickens (2). This alloantiserum can agglutinate erythrocytes, apparently by binding to the putative receptor encoded by tvbs1 in a complex with endogenous subgroup E viral envelope glycoprotein (2). Therefore, R2-specific agglutination served as a useful marker to follow the segregation of the tvbs1 allele from JF chickens among the East Lansing (Mich.) reference population, representing 52 F2 progeny of a backcross between a male (JF × WL) and WL females (5).
R2-specific agglutination of cells reflects a tvbs1-encoded cell polymorphism related to the R blood group antigen that has been mapped to East Lansing linkage group E38 (3b, 11). The E38 linkage group also contains an expressed sequence tag, com152e, that was first isolated from a chicken T-cell library (11). SacI RFLPs can distinguish between alleles of com152e in JF and WL chickens (11). RFLP analysis of the 52 backcross progeny revealed that the JF-specific tvbs1 allele (detected by R2 agglutination) always cosegregated with the JF-specific com152e allele (Table 1).
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To determine whether CAR1 mapped to the E38 linkage group, and thus to tvb, we attempted to identify nucleotide differences that distinguish the JF-specific and WL-specific alleles of this gene. DNA fragments containing an intron of CAR1, located between nucleotides (nt) 732 and 733 of the CAR1 cDNA clone (3, 3a), were isolated from WL and JF genomic samples by using a PCR-based approach that employed exon-specific oligonucleotide primers (Fig. 2). PCR products were cloned into the PCR 2.1 vector by using the TA cloning protocol (Invitrogen), and these DNA samples were sequenced by the dideoxy chain termination method by using an ABI model 373A automatic DNA sequencer.
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A comparison of DNA sequences revealed two nucleotide substitutions between the introns of the JF and WL alleles of CAR1. A C residue and a G residue in the WL allele were replaced by a G residue (nt 285) (Fig. 2) and an A residue (nt 379) (Fig. 2), respectively, in the JF allele (nt 379) (Fig. 2). Consequently, a reverse oligonucleotide primer mismatched at the 3' end (nt 285) (Fig. 2) with respect to the WL allele and another forward primer were used to generate a 209-bp DNA product that was amplified specifically from the intron of the JF allele (Fig. 2). Under the conditions used, the 209-bp DNA product was obtained only from JF and not WL chickens (Fig. 3, lanes J and W, respectively), and therefore the presence of this fragment could serve as a molecular marker to follow the segregation of the JF allele of CAR1 among the F2 backcross progeny.
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80°C.
To follow the segregation of the JF allele of CAR1, DNA from the 52 backcross progeny was analyzed by the PCR approach. Southern blot analysis with a radiolabeled, intron-containing DNA fragment derived from the BK9 CAR1 genomic DNA clone (3) identified those samples that contained the 209-bp DNA fragment (Fig. 3). In addition, fragments of this size derived from representative backcross progeny were subjected to DNA sequencing to validate the identity of the segregating allele (data not shown). These studies revealed that 25 of the 52 progeny contained the JF allele of CAR1 (samples 1, 6 to 9, 15 to 17, 19, 21 to 24, 27, 31 to 33, 35 to 38, 41, 47, 48, and 52) (Fig. 3). Although the signal observed with samples 7 and 9 appears weak, the presence of the 209-bp DNA fragment in these samples was confirmed independently by ethidium bromide staining of the PCR products following agarose gel electrophoresis (data not shown). Some of the amplified samples (e.g., samples 38 to 45) contained larger DNA fragments of approximately 500 bp that hybridized with the CAR1 intron probe (Fig. 3). These fragments were presumably derived from either the JF or WL alleles of CAR1 during the first step of PCR, which employed the outer oligonucleotide primer pair (Fig. 2).
Among these progeny, the JF alleles of CAR1, com152e, and tvb (defined by R2 agglutination) always cosegregated (Table 1). The lack of recombination between CAR1 and tvbs1 among progeny tested and the high LOD score (15.7) obtained with the Map Manager program have indicated that CAR1 and tvbs1 either are allelic or occur within 0.5 Mb. In the East Lansing linkage map, 1 centimorgan (1% recombination) represents a genetic distance of about 0.5 Mb (8). Because only three markers thus far have been mapped to linkage group E38, it appears likely that E38 represents one of the 30 chicken microchromosomes. Taken together, these data demonstrate that CAR1 maps to the chicken tvb locus and provide compelling evidence that this cloned gene is the s3 allele of tvb.
We are now attempting to isolate and characterize the single-copy CAR1 gene at tvbs1 (Fig. 1). This gene is predicted to encode a receptor for ALV-E in addition to those for ALV-B and ALV-D. Once this receptor has been identified, a comparison of its amino acid sequence with those of CAR1 (3) and SEAR (1) should help delineate ALV-B/D/E entry determinants of chicken Tvb proteins. A detailed analysis of these receptors should also help us understand how ALV-B(D)-receptor interactions apparently lead to cell death following infection, whereas ALV-E-receptor interactions do not (3, 6, 13, 14).
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ACKNOWLEDGMENTS |
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We thank Larry Bacon and Hans Cheng for helpful discussions. We also acknowledge the expert technical assistance of Cecyl Fischer and Laurie Molitor.
This research was supported, in part, by USDA-ARS Cooperative Agreement 58-3635-1-106 and by NIH grant CA 70810.
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FOOTNOTES |
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* Corresponding author. Mailing address: USDA Agricultural Research Service, Avian Disease and Oncology Lab, 3606 E. Mount Hope Rd., East Lansing, MI 48823. Phone: (517) 337-6828. Fax: (517) 337-6776. E-mail: Smitheu1{at}pilot.msu.edu.
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J Virol, April 1998, p. 3501-3503, Vol. 72, No. 4
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
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