# Reference Genes for Expression Analyses by qRT-PCR in Enterobacter cancerogenus

**Authors:** Yang Pan, Yue Zhao, Hua-Rui Zeng, Jia-Qi Wu, Ying-Ying Song, Ya-Hao Rao, Guo-Qing Li, Lin Jin

PMC · DOI: 10.3390/microorganisms12051024 · Microorganisms · 2024-05-19

## TL;DR

This study identifies optimal reference genes for qRT-PCR in Enterobacter cancerogenus to better analyze gene expression related to insect pathogenicity.

## Contribution

The study provides condition-specific reference gene combinations for accurate qRT-PCR normalization in entomopathogenic bacteria.

## Key findings

- gyrA and gyrB were the most stable reference genes across all tested conditions.
- Different reference gene combinations were optimal at different culture temperatures and bacterial OD values.
- Using gyrA and gyrB, the study showed high expression of Hcp in insect tissues, indicating a potential pathogenic role.

## Abstract

The Enterobacter cancerogenus strain EcHa1 was isolated from the dead larvae of Helicoverpa armigera, and has the potential for biocontrol of some Lepidoptera insects. In order to screen insecticidal-related genes by qRT-PCR, stable endogenous reference genes used for normalizing qRT-PCR data were selected and evaluated from 13 housekeeping genes (HKGs). The expression levels of the HKGs were determined using qRT-PCR under different experimental conditions, including two culture temperatures and three bacterial OD values. Five stability analysis methods (Ct, BestKeeper, NormFinder, geNorm, and RefFinder) were used to comprehensively rank the candidate genes. The results showed that the optimal reference genes varied under different experimental conditions. The combination of gyrA and gyrB was recommended as the best reference gene combination at 28 °C, while gyrA and rpoB was the best combination at 37 °C. When the OD values were 0.5, 1.0 and 2.0, the recommended reference gene combinations were ftsZ and gyrA, rpoB and gyrB, and gyrA and pyk, respectively. The most suitable reference genes were gyrA and gyrB under all experimental conditions. Using gyrA and gyrB as the reference genes for qRT-PCR, EcHa1 was found to invade all tissues of the H. armigera larvae, and expressed a candidate pathogenic factor Hcp at high levels in gut, Malpighian tubules, and epidermis tissues. This study not only establishes an accurate and reliable normalization for qRT-PCR in entomopathogenic bacteria but also lays a solid foundation for further study of functional genes in E. cancerogenus.

## Linked entities

- **Genes:** GYRA (DNA GYRASE A) [NCBI Gene 820238], gyrB (DNA gyrase subunit B) [NCBI Gene 857440], rpoB (RNA polymerase beta subunit) [NCBI Gene 800292], ftsZ (cell division protein FtsZ) [NCBI Gene 857456], PHKA2 (phosphorylase kinase regulatory subunit alpha 2) [NCBI Gene 5256], AMBP (alpha-1-microglobulin/bikunin precursor) [NCBI Gene 259]
- **Species:** Enterobacter cancerogenus (taxon 69218), Helicoverpa armigera (taxon 29058)

## Full-text entities

- **Species:** Enterobacter cancerogenus (species) [taxon 69218], Helicoverpa armigera (American bollworm, species) [taxon 29058]

## Full text

_Full body text omitted from this summary view._ Fetch the complete paper as Markdown: https://tomesphere.com/paper/PMC11123693/full.md

## Figures

8 figures with captions in the complete paper: https://tomesphere.com/paper/PMC11123693/full.md

## References

52 references — full list in the complete paper: https://tomesphere.com/paper/PMC11123693/full.md

---
Source: https://tomesphere.com/paper/PMC11123693