3′ BCR recombines with IGL locus in BCRABL–positive Philadelphia‐negative chronic myeloid leukemia

Benjes, Suzanne M.; Millow, Lynn J.; Jeffs, Aaron; Sowerby, Stephen J.; Reeve, Anthony E.; Morris, Christine M.

doi:10.1002/(sici)1098-2264(199912)26:4<366::aid-gcc11>3.3.co;2-o

Cited by 1 publication

(7 citation statements)

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“…The 6053 bp of DNA sequence, when submitted to BLASTN (http://www.ncbi.nlm.nih.gov/blast/blast.cgi, 5-4-01), was not present in the database but showed complete and intact alignment to various L1 elements. The L1 element polymorphism identified here was previously determined to map within the IGL locus (Benjes et al 1999) and therefore designated L1 IGL . L1 IGL showed highest homology to a full-length L1 element inserted into chromosome Y (bacterial artificial chromosome clone RP11-65E7, ACD10081-41/AC010081, nucleotides 19478-13446) and a full-length element inserted into the NOD1 gene on chromosome 7p14-p15 (AF149774.1/HSNOD1G2, nucleotides 12145-18160), with 99.58% and 99.54% nucleotide identities, respectively.…”

Section: Features Of the Inserted Segment Are Consistent With L1 Insementioning

confidence: 93%

“…Southern blot analysis of genomic DNA and polymerase chain reaction products High molecular weight DNA isolated from leukemic cells or peripheral blood (PB) cells from normal consenting donors was digested with restriction enzymes, electrophoresed, Southern-blotted, and hybridized with 32 P-dCTP-oligolabeled probes and methods previously described (Benjes et al 1999). Polymerase chain reaction (PCR) products were electrophoresed, Southern-blotted, and hybridized as for high-molecular-weight DNA.…”

Section: Methodsmentioning

confidence: 99%

“…2; Morris et al 1986). We have shown that the 3′ part of BCR has recombined at a site on chromosome 22 within the immunoglobulin lambda locus (IGL) intervening variable-gene region IV (Itv-Region IV), between two variable genes Vλ3-4 and Vλ5-4 (Benjes et al 1999). A genomic probe, initially used to confirm the authenticity of the cloned IGL/3′BCR breakpoint junction fragment and to isolate the corresponding IGL germline segment that spans the 3′BCR recombination site, detected an insertion polymorphism in normal control DNA.…”

Section: Suzanne M Benjes · Christine M Morrismentioning

confidence: 99%

“…A genomic probe, initially used to confirm the authenticity of the cloned IGL/3′BCR breakpoint junction fragment and to isolate the corresponding IGL germline segment that spans the 3′BCR recombination site, detected an insertion polymorphism in normal control DNA. Two allelic variants were identified that exhibited stable Mendelian inheritance and mapped ~3 kb 5′ of the IGL breakpoint (Benjes et al 1999). Here, we describe our molecular characterization of this polymorphic site and report the identification of a new and potentially active L1 element that maps within the IGL locus immediately upstream of BCR and within a wider region of chromosome 22q11.2 that is particularly prone to genomic instability associated with many inherited and malignant genetic conditions.…”

Section: Suzanne M Benjes · Christine M Morrismentioning

confidence: 99%

“…1a, probe c; Benjes et al 1999). To determine more specifically the insertion site of the identified insertion polymorphism, genomic DNA of individuals with genotypes A 1 A 1 , A 1 A 2 , and A 2 A 2 was digested with the enzymes BglII, BamHI, HindIII, and EcoRI and Southern-blotted.…”

Section: Molecular Refinement Of the Polymorphic Insertion Sitementioning

confidence: 99%

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A full-length and potentially active LINE element is integrated polymorphically within the IGL locus in a genomically unstable region of chromosome 22

Benjes¹,

Morris²

2001

Hum Genet

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Leukemic cells of a patient diagnosed with chronic myeloid leukemia (CML) showed a complex BCR-ABL1 rearrangement hidden within a normal appearing karyotype. Previous molecular studies had established that the 3' BCR had recombined at a novel site within the variable region of the immunoglobulin lambda locus ( IGL). A segment of DNA mapping very close to the site of the IGL/3' BCR recombination recognized a previously undescribed insertion polymorphism. A combination of molecular hybridization studies and long-range polymerase chain reaction was used to isolate a 6-kb full-length long interspersed nuclear element (LINE or L1), here designated L1(IGL), which occupies 19% of alleles in the general population. Although unclonable, DNA sequence analysis by a primer walking approach established that L1(IGL) has features characteristic of an actively retrotransposing element. The L1(IGL) element has a 5' untranslated region, two open reading frames (ORF-1 and ORF-2), a 3' untranslated region and terminates in a poly-A tail. We compared the DNA sequence and the predicted amino acid sequence of L1(IGL) with a consensus sequence compiled from seven reported active L1 elements. This analysis indicated that L1(IGL) has high potential for involvement in as yet undetermined somatically and constitutionally acquired disease, not only through recombination mechanisms, but also through retrotransposition events. This full-length L1 element maps close within the IGLlocus to L1.2, one of only nine active L1 elements that have been reported so far. L1(IGL) and L1.2 map within a wider and well-recognized region of genomic instability on chromosome 22.

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Section: Features Of the Inserted Segment Are Consistent With L1 Insementioning

confidence: 93%

Section: Methodsmentioning

confidence: 99%