Alternatively spliced mRNAs. (A) At least six forms of mRNA that differ by splicing arise from the YKL186C region. PCR products from genomic DNA (gDNA, lane 1) and RT–PCR products from cDNA (RNA, lane 2) are compared to marker DNA (lane M, 100 bp ladder marker, the fastest migrating band is 100 bp, next fastest is 200 bp, etc.). Positions of the two 5′ splice sites (labeled 1 and 2) and the three 3′ splice sites (labeled a–c) relative to YKL186C are shown on the unspliced RNA (un) to the right of the gel. Different spliced forms of YKL186C mRNA and the migration of the corresponding PCR products are indicated. From top: un, unspliced; 2-a, 5′ splice site 2 joined to 3′ splice site (3′ss) a; 1-a*, 5′ss 1 joined to 3′ss a; 2-b, 5′ss 2 joined to 3′ss b; 2-c, 5′ss 2 joined to 3′ss c; 1-b, 5′ss 1 joined to 3′ss b; 1-c, 5′ss 1 joined to 3′ss c. Shaded boxes indicate additional amino acids encoded at the N-terminus of the YKL186C coding sequence. Each spliced form is identified by sequence of cloned PCR products except for 1-a, as indicated by the asterisk. The numbers above exon segments refer to amino acids encoded, the numbers below the introns refer to nucleotides removed by splicing. (B) Two forms of spliced RNA from the YML034W region. A previously unannotated intron near the 3′ end of YML034W uses two different 5′ splice sites. Top, positions of YML034W and YML033W (white boxes); middle, use of the downstream 5′ss leads to fusion of most of the YML034W (white box) coding sequence to 48 amino acids plus the coding sequence of YML033W (black box); bottom, use of the upstream 5′ss leads to fusion of most of the YML034W coding sequence to a different 48 amino acids (gray box) encoded in a different reading frame.