DNA-mediated transformation in Neurospora crassa results in the formation of heterokaryons comprising a mixture of both transformed and untransformed nuclei. This makes it imperative to resolve the transformed nuclei from the untransformed ones. The present methods for purifying the transformed nuclei from primary transformants include repeated plating of macroconidial transformant to enrich the transformed nuclei or producing uninucleate microconidia. Both these methods are labour intensive and time consuming. We report here a simple and efficient method of purifying the transformed nuclei by the induction of microconidiation in an otherwise non-microconidiating strain using a mcm mutant strain

Dev, Kamal

Maheshwari, Ramesh

Fungal Genetics Reports

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Kansas State University

Fungal Genetics Reports Volume 48 Article 4 Use of mutant mcm strain in purification of Neurospora crassa transformants resistant to hygromycin Kamal Dev Indian Institute of Science Ramesh Maheshwari Indian Institute of Science Follow this and additional works at: https://newprairiepress.org/fgr This work is licensed under a Creative Commons Attribution-Share Alike 4.0 License. Recommended Citation Dev, K., and R. Maheshwari (2001) "Use of mutant mcm strain in purification of Neurospora crassa transformants resistant to hygromycin," Fungal Genetics Reports: Vol. 48, Article 4. https://doi.org/10.4148/1941-4765.1169 This Regular Paper is brought to you for free and open access by New Prairie Press. It has been accepted for inclusion in Fungal Genetics Reports by an authorized administrator of New Prairie Press. For more information, please contact cads@k-state.edu. Use of mutant mcm strain in purification of Neurospora crassa transformants resistant to hygromycin Abstract DNA-mediated transformation in Neurospora crassa results in the formation of heterokaryons comprising a mixture of both transformed and untransformed nuclei. This makes it imperative to resolve the transformed nuclei from the untransformed ones. The present methods for purifying the transformed nuclei from primary transformants include repeated plating of macroconidial transformant to enrich the transformed nuclei or producing uninucleate microconidia. Both these methods are labour intensive and time consuming. We report here a simple and efficient method of purifying the transformed nuclei by the induction of microconidiation in an otherwise non-microconidiating strain using a mcm mutant strain. This regular paper is available in Fungal Genetics Reports: https://newprairiepress.org/fgr/vol48/iss1/4 10 Fungal Genetics NewsletterUse of mutant mcm strain in purification of Neurospora crassa  transformants resistant to hygromycinKamal Dev and Ramesh Maheshwari.  Department of Biochemistry, Indian Institute of Science, Bangalore 560 012, India.DNA-mediated transformation in  Neurospora crassa  results in the formation of heterokaryons comprising a mixture ofboth transformed and untransformed nuclei. This makes it imperative to resolve the transformed nuclei from the untransformedones. The present methods for purifying the transformed nuclei from primary transformants include repeated plating ofmacroconidial transformant to enrich the transformed nuclei or producing uninucleate microconidia. Both these methods are labourintensive and time consuming.  We report here a simple and efficient method of purifying the transformed nuclei by the inductionof microconidiation in an otherwise non-microconidiating strain using a mcm mutant strain.______________________________________________________________________________                        Ever since the first successful report of genetic transformation in Neurospora crassa  (Mishra 1979 J. Gen.Microbiol. 133: 255-259), the technique has continuously improved.  Genetic transformation has been used as a tool to clone anumber of genes by complementation (Vollmer and Yanofsky 1986 Proc. Natl. Acad. Sci. U.S.A. 83: 4869-4873), as well as toreveal new phenomena such as RIP (Selker et al.1987 Cell 51: 741-752), and quelling (Romano and Macino 1992 Molec.Microbiol. 6: 3343-3353). Further studies have shown that competence for transformation is a nuclear rather than a cellularphenomenon (Grotelueschen and Metzenberg 1995 Genetics 139: 1545-1551 and Pandit and Russo 1992, Mol. Gen. Genet.234:412-422) and ectopic integration of transforming DNA was rare among transformants selected for gene replacement (Miao etal. 1995 Genetics 139: 1533-1534). Because of this property, the introduction of exogenous DNA results in the generation of aheterokaryon comprising a mixture of transformed and untransformed nuclei in the same cytoplasm. Such a heterogenous systemis less amenable for further studies and thus it becomes a prerequisite to obtain a homokaryotic transformant from theheterokaryon to carry out genetic and biochemical characterisation of the transformants.  Several methods have been developed topurify the transformant nuclei.                   One of the earliest methods involved the purification of the transformed nuclei by passing through a sexual cross, butthe method is generally unsuccessful because of the RIP phenomenon (Selker et al.1987 Cell 51: 741-752), which inactivates boththe ectopic and endogenous copies of the gene of interest. Alternatively, vegetative purification employs the use of multinucleatemacroconidia as well as the uninucleate microconidia. In case of macroconidia, purification of the transformed nuclei is done by alaborious method involving repeated plating of macroconidia of transformants and selecting for the transforming DNA phenotypefrom single macroconidial isolates.   Such isolates are then verified for the absence of the untransformed nuclei. An easierapproach, which includes looking for occasional homokaryons among random macroconidial isolates, has also been used.Uninucleate microconidia provide another alternative of purifying the transformants. Certain genotypes of N. crassa , e.g.,the fluffy strain of N. crassa  (FGSC 45), selectively produce only microconidia. This strain was transformed with a plasmidcarrying gene for the benomyl-resistance. The transformed strain was allowed to produce microconidia and individual(homokaryotic) transformed colonies were obtained. (Rossier et al. 1985 Curr. Genet.  10: 313-320).  Ebbole and Sachs (1990Fungal Genet. Newsl. 27:17-18), induced the primary transformant to produce microconidia which were then plated on selectivemedium to purify the transformed nuclei.  The availability of the mcm mutant (Maheshwari 1991 Exp. Mycol. 15: 346-350) and itsability to produce microconidia gave a major advantage over the previous methods. Since then, microconidia have been used inmany different ways to purify the transformed nuclei. A mcm mutant strain (Maheshwari 1991 Exp. Mycol. 15: 346-350) was usedto generate transformable spheroplasts (Royer and Yamashiro 1992 Fungal Genet. Newsl. 39: 76-77). The cellophane method(Pandit and Maheshwari, 1994 Fungal Genet. Newsl. 40: 64-65) was used to purify transformed nuclei from the untransformednuclei (Margolin et al. 1997 Fungal Genet. Newsl. 44: 43-36). In other cases the mcm gene has been incorporated in the parentstrain, so as to purify the transformed nuclei subsequently (Pitchaimani and Maheshwari 2000 Fungal Genet. Newsl. 47: 89-91).All these methods have their own limitations; for example, it is a time consuming process to introduce the fluffy or mcm gene intothe parent strain before transformation.  The transformation of microconidial spheroplasts is limited by their low viability (12%).Here we report the use of a mutant mcm strain to purify wild type N. crassa, which has been transformed with the hph gene.          Grigg (Neurospora Newsl. 7: 12-13) observed that a normal macroconidial strain could be induced to form microconidia ifcombined in a heterokaryon with a microconidial strain with the nuclear ratio (1:20 to 1: 40 respectively) in favour of themicroconidial strain.  We have used this observation to design a simple and efficient method to purify the transformed nuclei.  Wehave generated a heterokaryon by mixing the impure transformant with an excess of a het-compatible mcm strain containing aselection marker and growing the heterokaryon to conidiation.  Macroconidia from such a heterokaryon were shaken overnight toobtain microconidia and plated to isolate the transformed nucleus for hygromycin resistance in pure homokaryotic form. Thus, anotherwise non-microconidiating transformant is induced by the mcm counterpart to produce microconidia.1Dev and Maheshwari: Use of mutant mcm strain in purification of Neurospora crassa traPublished by New Prairie Press, 2017Number 48, 2001 11Generation of hygromycin resistance transformants: The wild type strain of N. crassa  OR23-I V A  (FGSC 2489) wastransformed by electroporation (Gene Pulsar II, BIORAD) with the plasmid pCSN44 containing the hph gene which encodes forhygromycin resistance (Staben et al. 1989 Fungal Genet. Newsl. 36: 79-81). Macroconidia from a week-old culture grown onVogel’s Medium N (Davis and de Serres 1970 Methods Enzymol. A17: 79-143) containing 1.5% (w/v) sucrose were harvested byusing sterile distilled water, and washed twice with 1M sorbitol. Approximately 1 × 108 conidia were mixed with 1µg of plasmidDNA in 40 µl of 1M sorbitol and electroporation was performed according to the method of Margolin et al. (Fungal Genet.Newsl., 44: 34-36). The electroporated macroconidia were plated on sorbose plating medium (Davis and de Serres 1970 MethodsEnzymol. A17: 79-143) without any selection pressure.  After 20 hrs of growth at 34°C, the plates were overlaid with soft agar(0.7% agar) supplemented with hygromycin B (Sigma Chemical Company, MO, USA) at a concentration of 150 µg/ml forselection of the hph+ transformants and further incubated at 34°C.  Transformant colonies started appearing after five days ofincubation, and they grew out of the soft agar. These colonies were transferred to slants of Vogel’s Medium N supplemented with1.5 % (w/v) sucrose and 150 µg/ml of hygromycin B.  Out of fifty colonies that were picked and subcultured, forty were found tobe hygromycin resistant. The presence of the transforming hph gene was confirmed by Southern analysis using linearised pCSN44as a probe (data not shown). The primary transformants confirmed by Southern analysis were used for the next step of purification.Purification of the primary transformant: To purify the hygromycin resistant transformants, a strain of N. crassa , al-1;mcm arg-5  was constructed using the following parent stocks: al-1 (JH 216, FGSC 3714); arg-5  (P9125), and mcm (RM124-2A,FGSC 7455).  Macroconidia of the constructed strain and that of the primary transformant were mixed in a ratio of 2:1respectively, and centrifuged to form a pellet.  The pellet was transferred to agar slants of Vogel’s Medium N with 1.5 % (w/v)sucrose and grown at 34°C to allow the formation of heterokaryon. After 7-10 days of growth, the macroconidia were harvestedand inoculated in liquid Vogel’s N Medium with 1.5 % (w/v) sucrose and grown at 22°C with shaking at 240 rpm to producemicroconidia. Abundant microconidia were produced because of the expression from the mcm mutant counterpart of theheterokaryon (Maheshwari 1991 Exp. Mycol. 15: 346-350). Since both the transformant nuclei and the mcm mutant nuclei share acommon cytoplasm in the heterokaryon, the mcm nuclei induce the microconidiation of the transformant nuclei as well(presumably through a diffusable factor). As a result, the microconidia formed would contain a mixed population of transformedand untransformed nuclei.The microconidia were separated from the germinated macroconidia by filtering the culture suspension through asynthetic fabric, ThermoLam Plus (Metzenberg 1989 Fungal Genet. Newsl. 36: 83) and plated on sorbose plating mediumcontaining 150 µg/ml hygromycin B.  After 24 hrs of growth at 34°C, another layer of soft agar containing hygromycin B (150µg/ml) was overlaid.  This would select only the homokaryotic hygromycin -resistant transformants.  Colonies appearing afterseven days were transferred to slants of Vogel’s Medium N with 1.5 % sucrose and 150 µg/ml of hygromycin B. The examinationof these purified cultures showed that they grew more vigorously as compared to the primary transformants. Moreover, thepurified transformants showed a higher tolerance to hygromycin (600 µg/ml) as compared to the primary transformants. Thepresence of the hph gene in these purified transformants was further confirmed by Southern analysis (not shown).This  simple and easy method can be used to purify primary transformant of any genotype without any further geneticmodification.Acknowledgement:  This work was supported by a grant from The Department of Biotechnology, Government of India, toRM.  We thank Keyur K. Adhvaryu for critical reading of the manuscript.2Fungal Genetics Reports, Vol. 48 [2001], Art. 4https://newprairiepress.org/fgr/vol48/iss1/4DOI: 10.4148/1941-4765.1169

Use of mutant mcm strain in purification of Neurospora crassa transformants resistant to hygromycin

Kamal Dev

Ramesh Maheshwari

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Use of mutant mcm strain in purification of Neurospora crassa transformants resistant to hygromycin

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