exRNAdisease

Entry Detail

General Information

Database ID:

exR0226440

RNA Name:

hsa-miR-500a-3p

RNA Type:

miRNA

Chromosome:

chrX

Starnd:

+

Coordinate:

Start Site(bp):

50008482

End Site(bp):

50008503

External Links:

hsa-miR-500a-3p

Disease Information

Disease Name:	Active Tuberculosis
Disease Category:	Infections
MeSH ID:	D014376
Type:	Diseases Category/Infections
Alias:	Tuberculosis//Tuberculoses//Kochs Disease//Koch's Disease//Koch Disease//Mycobacterium tuberculosis Infection//Infection, Mycobacterium tuberculosis//Infections, Mycobacterium tuberculosis//Mycobacterium tuberculosis Infections

Expression Detail

GEO ID:	GSE124120
Description:	Small RNA Profiles of Serum Exosomes Derived from Individuals with Latent and Active Tuberculosis
Experimental Design:	Disease vs Control
Case Disease Type:	Active Tuberculosis
Case Disease SubType:	NA
Case Sample:	Active Tuberculosis
Control Sample:	Healthy
Number of Case:	1
Number of Control:	1
Number of Samples:	2

Regulatory Relationship

mRNA targets:

NA

miRNA targets:

NA

circRNA targets:

circRNA Symbol	Chromosome	Start Site(bp)	End Site(bp)	Strand
hsa_circ_0001445	chr4	144464661	144465125	+

lncRNA targets:

lncRNA Symbol	Chromosome	Start Site(bp)	End Site(bp)	Strand
AC009133.5	chr16	29808679	29812227	+
AC016876.2	chr17	7581964	7584086	-
MIR17HG	chr13	91347820	91354579	+
MIR29B2CHG	chr1	207801518	207879115	-
NEAT1	chr11	65422774	65445540	+
NORAD	chr20	36045618	36051018	-
XIST	chrX	73820649	73852723	-

Display:

Experiment Detail

GEO ID:	GSE124120
Sample Source:	Blood
Source Fraction:	Exosome
Platform:	GPL16791
Method:	NGS
Num of detected RNA Type:	1
Num of detected RNAs of this Type:	356
Sample treatment protocol:	We first performed differential centrifugation (1000 g for 10 min at 4 °C, and 16,500 g for 30 min at 4 °C) to remove the cell debris, followed by ultrafiltration using 0.22 um filters. We then performed ultracentrifugation (120,000 g for 2 hours) to obtain exosome pellets. Transmission electron microscopy (TEM) was employed to visualize exosomes. The exosome pellets were first suspended and dropped onto 200 mesh copper grids, followed by incubation in 3% phosphotungstic acid for 10 min. The copper mesh was then washed three times with water and dried for observation by TEM. We also analyzed the exosome size distributions using the nanoparticle tracking analysis (NTA, Malvern, UK) according to the manufacturer's instructions.
RNA Extract protocol:	NA
RNA library preparation protocol:	Small RNA libraries were prepared for sequencing using standard Illumina protocols.

Reference

PMID:	https://doi.org/10.3389/fmicb.2019.01174
Title:	Small RNA Profiles of Serum Exosomes Derived From Individuals With Latent and Active Tuberculosis
Author:	Lingna Lyu, Xiuli Zhang, Cuidan Li, Tingting Yang, Jinghui Wang, Liping Pan, Hongyan Jia, Zihui Li, Qi Sun, Liya Yue, Fei Chen and Zongde Zhang
Journal:	Front. Microbiol., 28 May 2019 \| https://doi.org/10.3389/fmicb.2019.01174
Description:	In this study, we performed small RNA sequencing to explore small RNA profiles of serum exosomes derived from LTBI and TB patients and healthy controls (HC).