Utilization of Super BAC Pools and Fluidigm Access Array Platform for High-Throughput BAC Clone Identification: Proof of Concept

<table>Distribution of the SNP markers screened on linkage groups 1, 2, and 15 [<a href="/journals/bmri/2012/405940/#B22">22</a>]. Map distances are in cM, corrected with the Kosambi function.  SNP markers in the grey boxes were screened on the BAC library (<svg height="11.1625" id="M7" style="vertical-align:-0.27588pt" version="1.1" viewbox="0 0 42.912498 11.1625" width="42.912498" xmlns="http://www.w3.org/2000/svg">
<g transform="matrix(1.25,0,0,-1.25,0,11.1625)">
<g transform="translate(72,-63.07)">
<text transform="matrix(1,0,0,-1,-71.95,63.4)">
<tspan style="font-size: 12.50px; " x="0" y="0">𝑛</tspan>
<tspan style="font-size: 12.50px; " x="9.6773224" y="0">=</tspan>
<tspan style="font-size: 12.50px; " x="21.71771" y="0">9</tspan>
<tspan style="font-size: 12.50px; " x="27.969212" y="0">6</tspan>
</text>
</g>
</g>
</svg>).  BAC clones corresponding to SNP markers from LG2, indicated with a black arrow, were sequenced using 454-pyrosequencing.</table>

BioMed Research International

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Figure 2

Figure 2: Utilization of Super BAC Pools and Fluidigm Access Array Platform for High-Throughput BAC Clone Identification: Proof of Concept 