FIGURE

Fig. 1

ID
ZDB-FIG-160414-17
Publication
Mishima et al., 2016 - Codon Usage and 3' UTR Length Determine Maternal mRNA Stability in Zebrafish
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Fig. 1

Classification of Maternal mRNA Decay Pathways in Zebrafish

(A) A schematic representation of maternal mRNA decay pathways in zebrafish.

(B) Bright field pictures (upper panels) and in situ hybridization to detect gstm mRNA (lower panels, purple) in wild-type, miR-430 MO-injected, and α-amanitin-injected embryos.

(C) Left: a Venn diagram of the result of the RNA sequencing analysis. Right: pie charts representing subclasses of maternal genes whose mRNAs are degraded during MZT. The numbers show genes in each subclass.

(D) qRT-PCR analysis of wild-type and α-amanitin-injected embryos. mRNA levels at 0 hpf were set to one. The graph represents an average of three independent injection experiments. The error bars show SD.

(E) In situ hybridization to detect mRNAs of M-decay genes suv39h1a (upper panels) and pus1 (lower panels) in wild-type and α-amanitin-injected embryos. See also Figure S1.

Expression Data
Genes:
Fish:
Condition:
Knockdown Reagents:
Anatomical Term:
Stage Range: 1-cell to Shield

Expression Detail
Antibody Labeling
Phenotype Data
Fish:
Condition:
Knockdown Reagents:
Observed In:
Stage: Shield

Phenotype Detail
Acknowledgments
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