MAPPING DOMINANT MARKERS USING F2 MATINGS

被引:42
作者
KNAPP, SJ
HOLLOWAY, JL
BRIDGES, WC
LIU, BH
机构
[1] CLEMSON UNIV,DEPT EXPTL STAT,CLEMSON,SC 29634
[2] N CAROLINA STATE UNIV,DEPT FORESTRY,RALEIGH,NC 27695
关键词
BIAS; RECOMBINATION FREQUENCY; GENETIC MAPS; DNA MARKERS;
D O I
10.1007/BF00220861
中图分类号
S3 [农学(农艺学)];
学科分类号
0901 ;
摘要
The development of efficient methods for amplifying random DNA sequences by the polymerase chain reaction has created the basis for mapping virtually unlimited numbers of mixed-phase dominant DNA markers in one population. Although dominant markers can be efficiently mapped using many different kinds of matings, recombination frequencies and locus orders are often mis-estimated from repulsion F-2 matings. The major problem with these matings, apart from excessive sampling errors of recombination frequency (theta) estimates, is the bias of the maximum-likelihood estimator (MLE) of theta (theta(ML)). theta(ML) = 0 when the observed frequency of double-recessive phenotypes is 0 and the observed frequency of double-dominant phenotypes is less than 2/3 - the bias for those samples is - theta. We used simulation to estimate the mean bias of theta(ML). Mean bias is a function of n and theta and decreases as n increases. Valid maps of dominant markers can be built by using sub-sets of markers linked in coupling, thereby creating male and feamle coupling maps, as long as the maps are fairly dense (about 5 cM)- the sampling errors of theta increase as theta increases for coupling linkages and are equal to those for backcross matings when theta = 0. The use of F-2 matings for mapping dominant markers is not necessarily proscribed because they yield twice as many useful markers as a backcross population, albeit in two maps, for the same number of DNA extractions and PCR assays; however, dominant markers can be more effeciently exploited by using doubled-haploid, recombinant-inbred, or other inbred populations.
引用
收藏
页码:74 / 81
页数:8
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