I align RNA-seq reads to genome and then used cufflinks to do the assembly. But the output always skipped some regions for the gene call even though by IGV I could tell good alignments are existing there.


Here are the result lines from: genes.fpkm_trackingCUFF.1 - -
---------------------------
...

CUFF.10 - - CUFF.10 - - Scaffold1:111637-112521 - - 17.8444 13.9032 21.7856 OK
CUFF.11 - - CUFF.11 - - Scaffold1:114932-115447 - - 5.29068 2.10028 8.48108 OK
CUFF.12 - - CUFF.12 - - Scaffold1:117626-118329 - - 10.7109 7.14059 14.2812 OK
CUFF.13 - - CUFF.13 - - Scaffold1:116233-117155 - - 14.4199 10.9729 17.867 OK
CUFF.14 - - CUFF.14 - - Scaffold1:105973-107198 - - 76.2951 69.6545 82.9358 OK
CUFF.15 - - CUFF.15 - - Scaffold1:112755-114371 - - 93.4633 87.2185 99.708 OK
CUFF.16 - - CUFF.16 - - Scaffold1:114474-114851 - - 108.774 89.2379 128.311 OK
CUFF.17 - - CUFF.17 - - Scaffold1:27634-102622 - - 5567.72 5540.51 5594.93 OK
CUFF.18 - - CUFF.18 - - Scaffold1:618359-618942 - - 3.93266 1.44543 6.41989 OK
...
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The genes I am interested in are located at around 300k, but here there are only genes before 117k and after 618k

What should I do? Thanks