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by Honglin Chen, Paul Smith, Richard F. Ambinder, and S. Diane Hayward

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Presentation on theme: "by Honglin Chen, Paul Smith, Richard F. Ambinder, and S. Diane Hayward"— Presentation transcript:

1 by Honglin Chen, Paul Smith, Richard F. Ambinder, and S. Diane Hayward
Expression of Epstein-Barr Virus BamHI-A Rightward Transcripts in Latently Infected B Cells From Peripheral Blood by Honglin Chen, Paul Smith, Richard F. Ambinder, and S. Diane Hayward Blood Volume 93(9): May 1, 1999 ©1999 by American Society of Hematology

2 Illustration of the relative positions of the RPMS1, BARF0, and RK-BARF0 ORFs within BART transcripts and the location of the PCR primers used to detect RPMS1- and BARF0-containing cDNAs. Illustration of the relative positions of the RPMS1, BARF0, and RK-BARF0 ORFs within BART transcripts and the location of the PCR primers used to detect RPMS1- and BARF0-containing cDNAs. The sequence and coordinates of the primers are listed in Table 1. The 22.2 and RK1 cDNA clones have been previously reported.39 40 Honglin Chen et al. Blood 1999;93: ©1999 by American Society of Hematology

3 Specificity of the RT-PCR primers and oligonucleotide probes for EBER1, RPMS1, BARF0, and CD23.
Specificity of the RT-PCR primers and oligonucleotide probes for EBER1, RPMS1, BARF0, and CD23. RT-PCR and Southern blot analysis were performed as described in Materials and Methods. Raji is a human EBV+ lymphoblastoid cell line that expresses RPMS1, BARF0 and human CD23. B95-8 is a marmoset lymphoblastoid cell line that expresses simian CD23 and carries an EBV genome that is deleted in the BamHI-I region, which encodes RPMS1. Honglin Chen et al. Blood 1999;93: ©1999 by American Society of Hematology

4 Examination of EBNA-1 transcription in CD19+ PBMC by RT-PCR.
Examination of EBNA-1 transcription in CD19+ PBMC by RT-PCR. No EBNA-1 transcripts were detected in two CD19+ PBMC samples using primers specific for the EBNA-1 U-K splice, although EBER1 RNA was easily detectable. BJAB and B95-8 cells served as the negative and positive controls. Honglin Chen et al. Blood 1999;93: ©1999 by American Society of Hematology

5 Honglin Chen et al. Blood 1999;93:3026-3032
©1999 by American Society of Hematology

6 Honglin Chen et al. Blood 1999;93:3026-3032
©1999 by American Society of Hematology

7 Verification of the identity of the RPMS1 RT-PCR product.
Verification of the identity of the RPMS1 RT-PCR product. Alignment of an RPMS1 RT-PCR sequence cloned from a CD19+PBMC sample to known EBV sequences. The 5′ part of the sequence matched to Raji sequences spanning the B95-8 major deletion and the 3′ part of sequence matched B95-8 sequences as shown. Arrows indicate the splice sites and the numbers represent the positions in the Raji or B95-8 genome. Single-underlined sequences represent the primers used to generate the RT-PCR clone and the double-underlined 5 bp indicates an insertion relative to a reported cDNA.39The splice acceptor site (115,725) is the same as that seen in RK139 and the same sequence as that seen in C22.2,40 although there is a discrepancy in the numbering, which is given as 115,730 in Smith et al.40 Honglin Chen et al. Blood 1999;93: ©1999 by American Society of Hematology

8 Honglin Chen et al. Blood 1999;93:3026-3032
©1999 by American Society of Hematology

9 Honglin Chen et al. Blood 1999;93:3026-3032
©1999 by American Society of Hematology

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