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352236

Screening and Production of Fungal Arginine Degrading Enzymes and Testing Their Effects in Auxotrophic Cancers

Article

Last updated: 24 Dec 2024

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Tags

Basic Sciences

Abstract

The aim of the work: Finding and evaluating fungal arginine-degrading enzymes from various Egyptian soil habitats as anticancer mediators against auxotrophic cancer cells was the goal.
Methods: Fungal cultures that produced enzymes degrading arginine were subcultured on malt agar medium. The enzymes were then readily isolated after expression by salting out with ammonium sulfate and purified using anion exchange resin chromatography. Additionally, the evaluation of their auxotrophic anticancer properties in male rabbit animal models weighing close to 2 kg and several cancer cell lines. In this work, fungal arginine degrading enzymes were generated at pH 6.5, 25 °C, and incubation for three days using mineral arginine agar [MAM] selective medium [developed to select only fungi capable of using arginine as a single metabolic source of carbon and nitrogen].
Results: DNA blotting hybridization analyses identified Aspergillus as the primary fungal genus isolating these enzymes in the current investigation. Aspergillus fumigatus produced arginine decarboxylase and arginine deiminase, while Aspergillus niger was the producer of the L-arginase enzyme. They proved to be powerful anticancer drugs when used against these auxotrophic cancer cells. L-arginine amino acid is converted by arginine deiminase into Citrulline and ammonia. Ornithine and urea are produced from arginine by L-arginase. Extracellular proteins were identified as the enzymes degrading arginine. Based on spectrophotometric measurement of the Citrulline concentration and the ammonia concentration resulting from the hydrolysis of L-arginine by arginine deiminase, arginine deiminase synthesis and activity were examined. Using mass spectrometry and western blot-gel electrophoresis, the molecular masses of fungal L-arginase, arginine deiminase and arginine decarboxylase were determined to be 51 kDa, 53 kDa, and 37 kDa, respectively. L-arginase's Km and Vmax values were 8.63 mmol/l and 7.41 μmol/min, respectively.
Conclusion:  The study presented a unique fungal source of arginine-degrading enzymes from different soil conditions as anticancer mediators.

DOI

10.21608/ijma.2024.266915.1922

Keywords

FUNGAL, Arginine, Enzymes, Screening, Anticancer

Authors

First Name

Mohammed

Last Name

Kassab

MiddleName

M.

Affiliation

Department of Microbiology and Immunology, Faculty of Pharmacy, Cairo University, Giza, Egypt

Email

ksabmhmd676@gmail.com

City

cairo

Orcid

0000-0003-2554-0663

Volume

6

Article Issue

4

Related Issue

47405

Issue Date

2024-04-01

Receive Date

2024-01-31

Publish Date

2024-04-01

Page Start

4,293

Page End

4,309

Print ISSN

2636-4174

Online ISSN

2682-3780

Article File

IJMA_Volume 6_Issue 4_Pages 4293-4309.pdf

PDF . 2.3MB

Link

https://ijma.journals.ekb.eg/article_352236.html

Detail API

https://ijma.journals.ekb.eg/service?article_code=352236

Order

8

Type

Original Article

Type Code

816

Publication Type

Journal

Publication Title

International Journal of Medical Arts

Publication Link

https://ijma.journals.ekb.eg/

MainTitle

Screening and Production of Fungal Arginine Degrading Enzymes and Testing Their Effects in Auxotrophic Cancers

Details

Type

Article

Created At

24 Dec 2024