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. Author manuscript; available in PMC: 2013 Sep 1.

Published in final edited form as: Fertil Steril. 2012 Jun 19;98(3):713–719. doi: 10.1016/j.fertnstert.2012.05.027

Figure 1A. RT-PCR confirmed the expression of NGF mRNA (predicted amplicon=340 bp) and GAPDH mRNA (predicted amplicon=185 bp) in eutopic endometrial biopsies from two independent and representative controls (C) and two independent endometriosis (E) subjects. Amplicon lengths are indicated as base pairs (bp) and correspond with the molecular weight (MW) ladder in the left lane.

Figure 1B. RT-PCR confirmed the expression of BDNF mRNA (predicted amplicon=120 bp), NT-4/5 mRNA (predicted amplicon=96 bp) and GAPDH mRNA (predicted amplicon=185 bp) in eutopic endometrial biopsies from a representative control (C) and two independent endometriosis (E) subjects. GAPDH amplification was performed in duplicate. Molecular weight (MW) ladder is shown at left.

Figure 1A. RT-PCR confirmed the expression of NGF mRNA (predicted amplicon=340 bp) and GAPDH mRNA (predicted amplicon=185 bp) in eutopic endometrial biopsies from two independent and representative controls (C) and two independent endometriosis (E) subjects. Amplicon lengths are indicated as base pairs (bp) and correspond with the molecular weight (MW) ladder in the left lane.

Figure 1B. RT-PCR confirmed the expression of BDNF mRNA (predicted amplicon=120 bp), NT-4/5 mRNA (predicted amplicon=96 bp) and GAPDH mRNA (predicted amplicon=185 bp) in eutopic endometrial biopsies from a representative control (C) and two independent endometriosis (E) subjects. GAPDH amplification was performed in duplicate. Molecular weight (MW) ladder is shown at left.