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Mobile group II intron based gene targeting in Lactobacillus plantarum WCFS1

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The usage of recombinant lactic acid bacteria for delivery of therapeutic proteins to the mucosa has been emerging. In the present study, an attempt was made to engineer a thyA mutant of Lactobacillus plantarum (L. plantarum) using lactococcal group II intron Ll.LtrB for the development of biologically contained recombinant L. plantarum for prevention of calcium oxalate stone disease. The 3 kb Ll.LtrB intron donor cassettes from the source vector pACD4C was PCR amplified, ligated into pSIP series of lactobacillus vector pLp_3050sAmyA, yielding a novel vector pLpACD4C (8.6 kb). The quantitative real‐time PCR experiment shows 94‐fold increased expression of Ll.LtrB intron and 14‐fold increased expression of ltrA gene in recombinant L. plantarum containing pLpACD4C. In order to target the thyA gene, the potential intron RNA binding sites in the thyA gene of L. plantarum was predicted with help of computer algorithm. The insertion location 188|189s of thyA gene (lowest E‐0.134) was chosen and the wild type intron Ll.LtrB was PCR modified, yielding a retargeted intron of pLpACDthyA. The retargeted intron was expressed by using induction peptide (sppIP), subsequently the integration of intron in thyA gene was identified by PCR screening and finally ThyA− mutant of L. plantarum (ThyA18) was detected. In vitro growth curve result showed that in the absence of thymidine, colony forming units of mutant ThyA18 was decreased, whereas high thymidine concentration (10 μM) supported the growth of the culture until saturation. In conclusion, ThyA− mutant of L. plantarum (ThyA18) constructed in this study will be used as a biologically contained recombinant probiotic to deliver oxalate decarboxylase into the lumen for treatment of hyperoxaluria and calcium oxalate stone deposition.
Title: Mobile group II intron based gene targeting in Lactobacillus plantarum WCFS1
Description:
The usage of recombinant lactic acid bacteria for delivery of therapeutic proteins to the mucosa has been emerging.
In the present study, an attempt was made to engineer a thyA mutant of Lactobacillus plantarum (L.
plantarum) using lactococcal group II intron Ll.
LtrB for the development of biologically contained recombinant L.
plantarum for prevention of calcium oxalate stone disease.
The 3 kb Ll.
LtrB intron donor cassettes from the source vector pACD4C was PCR amplified, ligated into pSIP series of lactobacillus vector pLp_3050sAmyA, yielding a novel vector pLpACD4C (8.
6 kb).
The quantitative real‐time PCR experiment shows 94‐fold increased expression of Ll.
LtrB intron and 14‐fold increased expression of ltrA gene in recombinant L.
plantarum containing pLpACD4C.
In order to target the thyA gene, the potential intron RNA binding sites in the thyA gene of L.
plantarum was predicted with help of computer algorithm.
The insertion location 188|189s of thyA gene (lowest E‐0.
134) was chosen and the wild type intron Ll.
LtrB was PCR modified, yielding a retargeted intron of pLpACDthyA.
The retargeted intron was expressed by using induction peptide (sppIP), subsequently the integration of intron in thyA gene was identified by PCR screening and finally ThyA− mutant of L.
plantarum (ThyA18) was detected.
In vitro growth curve result showed that in the absence of thymidine, colony forming units of mutant ThyA18 was decreased, whereas high thymidine concentration (10 μM) supported the growth of the culture until saturation.
In conclusion, ThyA− mutant of L.
plantarum (ThyA18) constructed in this study will be used as a biologically contained recombinant probiotic to deliver oxalate decarboxylase into the lumen for treatment of hyperoxaluria and calcium oxalate stone deposition.

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