PMID- 12655496
OWN - NLM
STAT- MEDLINE
DCOM- 20030724
LR  - 20200930
IS  - 1552-4825 (Print)
IS  - 1552-4825 (Linking)
VI  - 118A
IP  - 2
DP  - 2003 Apr 15
TI  - SKY assessment of two karyotypes with 0-6 supernumerary marker/ring chromosomes 
      and review of previously reported cases with two or more markers.
PG  - 156-71
AB  - A 7-month-old boy with developmental delay and congenital abnormalities and a 
      58-year-old man with mental retardation, impaired speech, and dysmorphic features 
      were referred for cytogenetic studies. The peripheral blood chromosome studies of 
      Patient 1 had a de novo mosaic karyotype with 2-6 supernumerary marker 
      chromosomes. Patient 2 had a mosaic karyotype with 1-5 supernumerary marker 
      chromosomes and normal cells. All markers appeared to have a centromere by 
      C-banding and also by fluorescence in situ hybridization (FISH) using all 
      centromere probe for Patient 1. The majority of the markers appeared like rings. 
      Except for one marker in Patient 1 and 2-3 markers in Patient 2 with discernible 
      >5 Mb euchromatin, the rest of the markers were minute and some appeared to have 
      barely discernible euchromatin in C-banding or FISH. Spectral karyotyping (SKY) 
      was attempted to determine the origin of the marker chromosomes. Because some 
      markers had barely any euchromatin, their classification was not clear cut and 
      they were identified as derived from more than one chromosome. The SKY 
      classification of the markers in Patient 1 was 1, 3, 5, 7, 11, 15, and 22 and in 
      Patient 2 was 1, 5, 6, or 7. Patient 2 was lost to further follow-up studies. To 
      confirm the recurring SKY classifications in Patient 1, centromere probes for 
      chromosomes 1, 3, 5, 7, 11, 15, and 22 were used. The markers were negative for 
      1, 3, and 11 but positive for 7, 15, and 22 and probably 5. Since 5 centromere 
      probe cross hybridizes with 1 and 19, the weak signal on the marker/s in 
      successive hybridization did not give a definitive answer. Also, the 5 paint 
      probe was not conclusive because of the minute size of the marker. In some 
      metaphases, two markers were derived from 5 or 22. For clinical considerations, 
      the marker derived from 7, although variable in size, appeared to consistently 
      have euchromatin, followed by 15, while 22 and 5 markers were mostly centromeric 
      heterochromatin. The elastin gene probe that maps to 7q11.23, SNRPN gene that 
      maps to 15q11.2, and TUPLE gene that maps to 22q11.2 did not give a signal on the 
      markers. As expected for a majority of ring chromosomes, the pan telomere probe 
      did not hybridize to any of the markers. This highly unusual karyotype was 
      confirmed in the buccal epithelium using a mix of centromere 7 and 15 probes and 
      the combination 14/22 probe. The ratio of additional FISH signals in the buccal 
      mucosal cells was comparable to the ratios observed in the peripheral blood. In 
      this study, we have attempted to consolidate the data on >/=2 marker cases to 
      understand the analysis constraints, the range of clinical abnormalities, and the 
      mechanisms involved. The literature was surveyed for multiple markers cases. A 
      majority of the reported cases had two markers, either derived from the same 
      chromosome or from two different chromosomes or two cell lines with different 
      markers derived from the same chromosome. Cases with three or more markers were 
      rare. The nature and extent of euchromatin content of the multiple markers 
      appears to determine the phenotype. Frequently, multiple marker cases had small 
      to minute markers. The clinical presentation varied from mild to severe. While 
      two bisatellited markers may be associated with infertility, the phenotype in 
      other cases ranged from borderline intelligence and mild dysmorphism to 
      developmental delay, mental retardation, and congenital abnormalities.
CI  - Copyright 2003 Wiley-Liss, Inc.
FAU - Reddy, Kavita S
AU  - Reddy KS
AD  - Department of Cytogenetics, Quest Diagnostics, Inc., San Juan Capistrano, 
      California, USA. iamreddy@cox.net
FAU - Wang, Shirong
AU  - Wang S
FAU - Groh, Shannon
AU  - Groh S
FAU - Gonatos, John
AU  - Gonatos J
LA  - eng
PT  - Case Reports
PT  - Journal Article
PT  - Review
PL  - United States
TA  - Am J Med Genet A
JT  - American journal of medical genetics. Part A
JID - 101235741
SB  - IM
MH  - *Aneuploidy
MH  - Chromosome Banding
MH  - Chromosomes, Human, Pair 22/genetics
MH  - Chromosomes, Human, Pair 5/genetics
MH  - Chromosomes, Human, Pair 7/genetics
MH  - Humans
MH  - In Situ Hybridization, Fluorescence
MH  - Infant
MH  - Karyotyping/methods
MH  - Male
MH  - Middle Aged
MH  - *Ring Chromosomes
MH  - Trisomy
RF  - 79
EDAT- 2003/03/26 05:00
MHDA- 2003/07/25 05:00
CRDT- 2003/03/26 05:00
PHST- 2003/03/26 05:00 [pubmed]
PHST- 2003/07/25 05:00 [medline]
PHST- 2003/03/26 05:00 [entrez]
AID - 10.1002/ajmg.a.10045 [doi]
PST - ppublish
SO  - Am J Med Genet A. 2003 Apr 15;118A(2):156-71. doi: 10.1002/ajmg.a.10045.