Name: 4d microscopy of yeast
Uploaded: 2019-04-28T13:00:00
Description: Watch this Scientific Journal Video about 4D Microscopy of Yeast at JoVE.com

इस काम NIH अनुदान R01 GM104010 द्वारा समर्थित किया गया था. एकीकृत माइक्रोस्कोपी कोर सुविधा है, जो NIH वित्त पोषित कैंसर केंद्र सहायता अनुदान P30 CA014599 द्वारा समर्थित है पर Vytas Bindokas और क्रिस्टीन Labno को फ्लोरोसेंट माइक्रोस्कोपी के साथ सहायता के लिए धन्यवाद.

1. तैयारी
<ol><li>Nonfluorescent न्यूनतम NSD मध्यम2बनाओ | राइबोफ्लेविन की अनुपस्थिति से पृष्ठभूमि इंट्रासेल्यूलर ग्रीन फ्लोरोसेंट और संबद्ध फोटोटॉक्सिसिटी को कम करने की उम्मीद है।</li>
	<li>5 एमएल एनएसडी में 5 एमएल एनए?...

<ol>
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W., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+role+for+actin,+Cdc1p+and+Myo2p+in+the+inheritance+of+late+Golgi+elements+in+Saccharomyces+cerevisiae.">A role for actin, Cdc1p and Myo2p in the inheritance of late Golgi elements in Saccharomyces cerevisiae.</a> Journal of Cell Biology. 153 (1), 47-61 (2001).</li><li>Connerly, P. L., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Sec16+is+a+determinant+of+transitional+ER+organization.">Sec16 is a determinant of transitional ER organization.</a> Current Biology. 15 (16), 1439-1447 (2005).</li><li>Genov&#233;, G., Glick, B. S., Barth, A. L. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Brighter+reporter+genes+from+multimerized+fluorescent+proteins.">Brighter reporter genes from multimerized fluorescent proteins.</a> BioTechniques. 39 (6), 814-822 (2005).</li><li>Pawley, J. B. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=.">.</a> Handbook of Biological Confocal Microscopy. 3rd edn. , (2006).</li><li>Ishii, M., Suda, Y., Kurokawa, H., Nakano, A. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=COPI+is+essential+for+Golgi+cisternal+maturation+and+dynamics.">COPI is essential for Golgi cisternal maturation and dynamics.</a> Journal of Cell Science. 129 (17), 3251-3261 (2016).</li><li>Liss, V., Barlag, B., Nietschke, M., Hensel, M. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Self-labelling+enzymes+as+universal+tags+for+fluorescence+microscopy,+super-resolution+microscopy+and+electron+microscopy.">Self-labelling enzymes as universal tags for fluorescence microscopy, super-resolution microscopy and electron microscopy.</a> Scientific Reports. 5, 17740 (2015).</li><li>Grimm, J. B., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=A+general+method+to+improve+fluorophores+for+live-cell+and+single-molecule+microscopy.">A general method to improve fluorophores for live-cell and single-molecule microscopy.</a> Nature Methods. 12 (3), 244-250 (2015).</li><li>Casler, J. C., et al. <a target="_blank" href="http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?db=PubMed&cmd=Search&doptcmdl=Citation&defaultField=Title+Word&term=Maturation-driven+transport+and+AP-1-dependent+recycling+of+a+secretory+cargo+in+the+Golgi.">Maturation-driven transport and AP-1-dependent recycling of a secretory cargo in the Golgi.</a> Journal of Cell Biology. , (2019).</li></ol>

खमीर organelles के 4D confocal इमेजिंग कई मापदंडों के सावधान ट्यूनिंग की आवश्यकता है। प्रमुख चिंता photobleaching और phototoxicity है. एक ठेठ 4D फिल्म ऑप्टिकल वर्गों के हजारों इकट्ठा शामिल है, तो लेजर रोशनी के रूप में संभव के रूप में कम ?...

एंडोमेम्ब्रेन सिस्टम के कंपार्टमेंट्स लगातार फ्रलक्स में होते हैं, और उनकी पूर्ण विशेषता को लाइव सेल इमेजिंग की आवश्यकता होती है। यहाँ वर्णित एक प्रोटोकॉल है कि रोजगार 4D (समय चूक 3 डी) confocal माइक्रोस्कोपी नवोदित खमीर में फ्लोरोसेंट लेबल डिब्बों कल्पना है. इस विधि को पिकिया पासारिस और सकहोमोमिक्स सेरेविसे1,2,3में स्रावी डिब्बों की गतिशीलता को ट्रैक करने के लिए विकसित किया गया था . इस प्रोटोकॉल एस सेरेविसियाई पर केंद्रित है, जिसमें एक nonstacked Golgi है जिसमें व्यक्तिगत कुंडी ऑप्टिकली resolvable4हैं. एस सेरेविएसिया में असामान्य Golgi संगठन 4D माइक्रोस्कोपी द्वारा प्रदर्शन सक्षम है कि एक Golgi cisterna शुरू में निवासी जल्दी Golgi प्रोटीन के साथ लेबल, और फिर उन प्रोटीन खो देता है, जबकि निवासी देर Golgi प्रोटीनप्राप्त 3 ,5. इस संक्रमण एक तनाव है जिसमें जल्दी Golgi प्रोटीन Vrg4 GFP के साथ लेबल है, जबकि देर Golgi प्रोटीन Sec7 एक monomeric लाल फ्लोरोसेंट प्रोटीन के साथ लेबल है बनाने के द्वारा कल्पना की जा सकती है. जब अलग-अलग कुंडों को ट्रैक किया जाता है, तो परिपक्वता को हरे-से-लाल रूपांतरण3के रूप में देखा जाता है। विश्लेषण के इस प्रकार प्रोटीन स्थानीयकरण और डिब्बे पहचान के बारे में बहुमूल्य जानकारी प्रदान कर सकते हैं. उदाहरण के लिए, थोड़ा ऑफसेट आगमन और प्रस्थान समय के साथ दो प्रोटीन कभी कभी स्थिर छवियों में विभिन्न डिब्बों लेबल प्रकट हो सकता है, लेकिन 4D फिल्मों में देखा जा सकता है अलग अलग समय अंक6,7 पर एक ही डिब्बे लेबल . इस प्रकार, 4D माइक्रोस्कोपी घटना है कि अन्यथा स्पष्ट नहीं होगा पता चलता है.
खमीर डिब्बों की जानकारीपूर्ण 4D माइक्रोस्कोपी उचित प्रक्रियाओं और उपकरण2के साथ प्राप्त किया जा सकता है। जब भी संभव हो, फ्लोरोसेंट प्रोटीन टैगिंग जीन प्रतिस्थापन8 द्वारा किया जाता है overexpression कलाकृतियों से बचने के लिए. क्योंकि intracellular संरचनाओं अक्सर बहुत गतिशील हैं, 4D इमेजिंग सुनिश्चित करें कि एक संरचना समय के साथ मज़बूती से ट्रैक किया जाता है की जरूरत है. यहाँ वर्णित प्रोटोकॉल उच्च संवेदनशीलता डिटेक्टरों से लैस एक लेजर स्कैनिंग confocal माइक्रोस्कोप कार्यरत हैं. इस डिवाइस के साथ, एस cerevisiae की पूरी सेल मात्रा confocal माइक्रोस्कोपी द्वारा लगभग हर 1-3 s द्वारा छवि बनाई जा सकती है, 2 s अंतराल के साथ विशिष्ट जा रहा है. फ्लोरोफोर्स के लेबलिंग घनत्व और उनके फोटोफिजिकल गुणों के आधार पर 5-15 मिनट तक डेटा एकत्र किया जा सकता है। मुख्य बाधा photobleaching को कम करने के लिए है। इस उद्देश्य के लिए, लेजर तीव्रता के रूप में संभव के रूप में कम रखा जाता है, confocal स्कैन गति अधिकतम है, और ऑप्टिकल पैरामीटर के लिए प्रासंगिक जानकारी पर कब्जा करने के क्रम में NyQuist सीमा पर छवि के लिए कॉन्फ़िगर कर रहे हैं, जबकि अत्यधिक प्रकाश जोखिम से परहेज. इन सेटिंग्स को भी phototoxicity को कम करने की उम्मीद कर रहे हैं, एक कारक है कि अक्सर लाइव सेल इमेजिंग9,10,11 केदौरान अनदेखी की है . परिणामस्वरूप शोर डेटा ब्लीच सुधार और deconvolution एल्गोरिदम के साथ संसाधित कर रहे हैं फ्लोरोसेंट तीव्रता के परिमाण की सुविधा के लिए.
यहां तक कि उच्च गुणवत्ता 4D फिल्मों के साथ, विश्लेषण मुश्किल है क्योंकि खमीर डिब्बों के लिए कई हो जाते हैं, विषम, और मोबाइल. confocal माइक्रोस्कोपी की आंतरिक सीमाओं और लंबे समय तक 4D इमेजिंग के लिए आवश्यक गैर इष्टतम सेटिंग्स के कारण, फ्लोरोसेंट संरचनाओं है कि एक दूसरे के पास हैं हल करने के लिए मुश्किल कर रहे हैं. इस समस्या को फ्लोरोसेंट संरचनाओं की छोटी संख्या पर ध्यान केंद्रित करके दरकिनार किया जा सकता है जो लेबलिंग अवधि की अवधि के लिए ऑप्टिकली समाधान योग्य रहते हैं, इस धारणा के साथ कि उन संरचनाओं लेबल की पूरी आबादी के प्रतिनिधि हैं डिब्बों. फ्लोरिसेंट डिब्बों कि मज़बूती से ट्रैक किया जा सकता है प्रक्षेपित की फिल्मों को देखने के द्वारा की पहचान कर रहे हैं - stacks और montages की एक श्रृंखला है जिसमें प्रत्येक समय बिंदु के लिए ऑप्टिकल वर्गों एक कंप्यूटर स्क्रीन पर arrayed हैं बनाने के द्वारा. इस विश्लेषण कस्टम ImageJ12 plugins है, जो एक व्यक्तिगत संरचना अलगाव में ट्रैक किया जा करने की अनुमति कार्यरत हैं.
हाल के तरीकों के कागजात खमीर13 में फ्लोरोसेंट प्रोटीन के उपयोग के साथ ही सिद्धांत और खमीर कोशिकाओं के 4D confocal इमेजिंग के अभ्यास को कवरकिया 2. इस प्रोटोकॉल एक 4D इमेजिंग प्रयोग के प्रमुख व्यावहारिक पहलुओं पर केंद्रित है. यह पहले से वर्णित प्रक्रियाओं, साथ ही ImageJ प्लगइन कोड और प्रलेखन के अद्यतन संस्करणों के लिए कुछ एन्हांसमेंट्स शामिल हैं. दिखाया उदाहरण Golgi गतिशीलता पर केंद्रित है, लेकिन इस प्रोटोकॉल अन्य खमीर डिब्बों इमेजिंग के लिए समान रूप से उपयुक्त है.

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		<tr height="42">
			<td height="42" style="height:42px;width:216px;">35 mm glass bottom dishes No. 1.5</td>
			<td style="width:85px;">MatTek</td>
			<td style="width:119px;">P35G-0.170-14-C</td>
			<td style="width:167px;">Imaging dishes</td>
		</tr>
		<tr height="42">
			<td height="42" style="height:42px;width:216px;">Concanavalin A powder</td>
			<td style="width:85px;">Sigma-Aldrich</td>
			<td style="width:119px;">C2010</td>
			<td></td>
		</tr>
		<tr height="63">
			<td height="63" style="height:63px;width:216px;">Trolox</td>
			<td style="width:85px;">Vector Laboratories</td>
			<td style="width:119px;">CB-1000</td>
			<td></td>
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		<tr height="63">
			<td height="63" style="height:63px;width:216px;">Leica SP8 confocal microscope</td>
			<td style="width:85px;">Leica Microsystems</td>
			<td style="width:119px;"></td>
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			<td height="63" style="height:63px;width:216px;">Leica Application Suite X&#160;</td>
			<td style="width:85px;">Leica Microsystems</td>
			<td style="width:119px;"></td>
			<td>Microscope software</td>
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		<tr height="63">
			<td height="63" style="height:63px;width:216px;">Huygens Essential software, version 17.04</td>
			<td style="width:85px;">Scientific Volume Imaging</td>
			<td style="width:119px;"></td>
			<td>Deconvolution software</td>
		</tr>
		<tr height="21">
			<td height="21" style="height:21px;width:216px;">ImageJ</td>
			<td style="width:85px;">NIH</td>
			<td style="width:119px;"></td>
			<td>Image processing and analysis software</td>
		</tr>
	</tbody>
</table>

4d microscopy of yeast

इस प्रोटोकॉल का लक्ष्य यह विशेषता है कि झिल्ली के डिब्बे कैसे बनते हैं और नवोदित खमीर की जीवित कोशिकाओं में बदलना है। खमीर में कई intracellular डिब्बों गतिशील हैं, और उनके गुणों की एक पूरी समझ समय चूक इमेजिंग की आवश्यकता है. बहु रंग 4D confocal फ्लोरोसेंट माइक्रोस्कोपी 5-15 मिनट के एक समय पैमाने पर एक intracellular डिब्बे के व्यवहार और संरचना पर नज़र रखने के लिए एक शक्तिशाली तरीका है. डिब्बे गतिशीलता के कठोर विश्लेषण ऑप्टिकल के हजारों की कब्जा की आवश्यकता है अनुभागों. इस उद्देश्य को प्राप्त करने के लिए, photobleaching और phototoxicity बहुत कम लेजर शक्ति पर तेजी से स्कैनिंग से कम कर रहे हैं, और पिक्सेल आयाम और जेड कदम अंतराल सबसे बड़ा मूल्यों है कि पूर्ण संकल्प पर छवि नमूना के साथ संगत कर रहे हैं करने के लिए सेट कर रहे हैं. परिणामस्वरूप 4D डेटा सेट शोर कर रहे हैं, लेकिन deconvolution द्वारा smoothed किया जा सकता है. यहां तक कि उच्च गुणवत्ता वाले डेटा के साथ, विश्लेषण चरण चुनौतीपूर्ण है क्योंकि इंट्रासेल्यूलर संरचनाएं अक्सर कई, विषम, और मोबाइल होती हैं। इस जरूरत को पूरा करने के लिए, कस्टम ImageJ plugins एक कंप्यूटर स्क्रीन पर सरणी 4D डेटा के लिए लिखा गया था, ब्याज की संरचनाओं की पहचान, व्यक्तिगत संरचनाओं को अलग करने के लिए डेटा संपादित करें, फ्लोरोसेंट समय पाठ्यक्रम मात्रा, और अनुमानित की फिल्में बनाने के लिए -stacks. 4D फिल्में विशेष रूप से क्षणिक डिब्बों कि परिपक्वता से अधिक बारी से स्थिर डिब्बों भेद के लिए उपयोगी होते हैं. इस तरह की फिल्मों को भी इस तरह के डिब्बे संलयन के रूप में घटनाओं की विशेषता के लिए इस्तेमाल किया जा सकता है, और विशिष्ट उत्परिवर्तनों या अन्य क्षोभ के प्रभाव का परीक्षण करने के लिए.

यहाँ दिए गए उदाहरण दस्तावेजों और दो खमीर Golgi cisterae की परिपक्वता के रूप में दोहरी रंग 4D confocal माइक्रोस्कोपी3द्वारा कल्पना की मात्रा निर्धारित करता है. एक खमीर सेल 10-15 Golgi cisterae के आदेश पर शामिल ...

Watch this Scientific Journal Video about 4D Microscopy of Yeast at JoVE.com

4D Microscopy of Yeast

खमीर की 4D माइक्रोस्कोपी

इस प्रोटोकॉल बहु रंग 4 डी (समय चूक 3 डी) confocal माइक्रोस्कोपी का उपयोग कर नवोदित खमीर में फ्लोरोसेंट लेबल intracellular डिब्बों के विश्लेषण का वर्णन करता है। इमेजिंग पैरामीटर photodamage सीमित करते समय पर्याप्त संकेतों पर कब्जा करने के लिए चुना जाता है. कस्टम ImageJ plugins लेबल संरचनाओं पर नज़र रखी और मात्रात्मक विश्लेषण किया जा करने के लिए अनुमति देते हैं.

The goal of this protocol is to characterize how membrane compartments form and transform in live cells of budding yeast. Many intracellular compartments ...

Research

JoVE Journal

Biology

Purification of Mitochondria from Yeast Cells

Mitochondria are the main site of ATP production during aerobic metabolism in eukaryotic non-photosynthetic cells1. These complex organelles also play essential roles in apoptotic cell death2, cell survival3, mammalian development4, neuronal development and function4, intracellular signalling5, and longevity regulation6. Our understanding of these complex biological processes controlled by mitochondria relies on robust methods for assessing their morphology, their protein and lipid composition, the integrity of their DNA, and their numerous vital functions. The budding yeast Saccharomyces cerevisiae, a genetically and biochemically manipulable unicellular eukaryote with annotated genome and well-defined proteome, is a valuable model for studying the molecular and cellular mechanisms underlying essential biological functions of mitochondria. For these types of studies, it is crucial to have highly pure mitochondria. Here we present a detailed description of a rapid and effective method for purification of yeast mitochondria. This method enables the isolation of highly pure mitochondria that are essentially free of contamination by other organelles and retain their structural and functional integrity after their purification. Mitochondria purified by this method are suitable for cell-free reconstitution of essential mitochondrial processes and can be used for the analysis of mitochondrial structure and functions, mitochondrial proteome and lipidome, and mitochondrial DNA.

We describe a rapid and effective method for purification of mitochondria from the yeast Saccharomyces cerevisiae. This method enables the high-yield isolation of pure mitochondria that are essentially free of contamination by other organelles and retain their structural and functional integrity after their purification.

Mitochondria के खमीर कक्ष से शोधन

Mitochondria are the main site of ATP production during aerobic metabolism in eukaryotic non-photosynthetic cells1. These complex organelles also play ...

Time-lapse Imaging of Mitosis After siRNA Transfection

Changes in cellular organization and chromosome dynamics that occur during mitosis are tightly coordinated to ensure accurate inheritance of genomic and cellular content. Hallmark events of mitosis, such as chromosome movement, can be readily tracked on an individual cell basis using time-lapse fluorescence microscopy of mammalian cell lines expressing specific GFP-tagged proteins. In combination with RNAi-based depletion, this can be a powerful method for pinpointing the stage(s) of mitosis where defects occur after levels of a particular protein have been lowered. In this protocol, we present a basic method for assessing the effect of depleting a potential mitotic regulatory protein on the timing of mitosis. Cells are transfected with siRNA, placed in a stage-top incubation chamber, and imaged using an automated fluorescence microscope. We describe how to use software to set up a time-lapse experiment, how to process the image sequences to make either still-image montages or movies, and how to quantify and analyze the timing of mitotic stages using a cell-line expressing mCherry-tagged histone H2B. Finally, we discuss important considerations for designing a time-lapse experiment. This strategy is complementary to other approaches and offers the advantages of 1) sensitivity to changes in kinetics that might not be observed when looking at cells as a population and 2) analysis of mitosis without the need to synchronize the cell cycle using drug treatments. The visual information from such imaging experiments not only allows the sub-stages of mitosis to be assessed, but can also provide unexpected insight that would not be apparent from cell cycle analysis by FACS.

Here we describe a basic protocol to image and quantify the mitotic timing of live mammalian tissue culture cells after siRNA transfection.

SiRNA अभिकर्मक के बाद समय चूक सूत्रीविभाजन की इमेजिंग

Changes in cellular organization and chromosome dynamics that occur during mitosis are tightly coordinated to ensure accurate inheritance of genomic and ...

Yeast Colony Embedding Method

Patterning of different cell types in embryos is a key mechanism in metazoan development. Communities of microorganisms, such as colonies and biofilms also display patterns of cell types. For example, in the yeast S. cerevisiae, sporulated cells and pseudohyphal cells are not uniformly distributed in colonies. The functional importance of patterning and the molecular mechanisms that underlie these patterns are still poorly understood.
One challenge with respect to investigating patterns of cell types in fungal colonies is that unlike metazoan tissue, cells in colonies are relatively weakly attached to one another. In particular, fungal colonies do not contain the same extensive level of extracellular matrix found in most tissues . Here we report on a method for embedding and sectioning yeast colonies that reveals the interior patterns of cell types in these colonies. The method can be used to prepare thick sections (0.5 &mu;) useful for light microscopy and thin sections (0.1 &mu;) suitable for transmission electron microscopy. Asci and pseudohyphal cells can easily be distinguished from ovoid yeast cells by light microscopy , while the interior structure of these cells can be visualized by EM.
The method is based on surrounding colonies with agar, infiltrating them with Spurr's medium, and then sectioning. Colonies with a diameter in the range of 1-2 mm are suitable for this protocol. In addition to visualizing the interior of colonies, the method allows visualization of the region of the colony that invades the underlying agar.

A method for embedding yeast colonies allowing sectioning for light and electron microscopy. This protocol allows determination of the distribution of sporulated cells and pseudohyphal cells within colonies providing a new tool toward understanding the organization of cell types within a fungal community.

खमीर कालोनी एम्बेडिंग विधि

Patterning of  different cell types in embryos is a key mechanism in metazoan development. Communities of microorganisms, such as colonies and biofilms ...

A Fluorescence Microscopy Assay for Monitoring Mitophagy in the Yeast Saccharomyces cerevisiae

Autophagy is important for turnover of cellular components under a range of different conditions. It serves an essential homeostatic function as well as a quality control mechanism that can target and selectively degrade cellular material including organelles1-4. For example, damaged or redundant mitochondria (Fig. 1), not disposed of by autophagy, can represent a threat to cellular homeostasis and cell survival. In the yeast, Saccharomyces cerevisiae, nutrient deprivation (e.g., nitrogen starvation) or damage can promote selective turnover of mitochondria by autophagy in a process termed mitophagy 5-9.
We describe a simple fluorescence microscopy approach to assess autophagy. For clarity we restrict our description here to show how the approach can be used to monitor mitophagy in yeast cells. The assay makes use of a fluorescent reporter, Rosella, which is a dual-emission biosensor comprising a relatively pH-stable red fluorescent protein linked to a pH-sensitive green fluorescent protein. The operation of this reporter relies on differences in pH between the vacuole (pH ~ 5.0-5.5) and mitochondria (pH ~ 8.2) in living cells. Under growing conditions, wild type cells exhibit both red and green fluorescence distributed in a manner characteristic of the mitochondria. Fluorescence emission is not associated with the vacuole. When subjected to nitrogen starvation, a condition which induces mitophagy, in addition to red and green fluorescence labeling the mitochondria, cells exhibit the accumulation of red, but not green fluorescence, in the acidic vacuolar lumen representing the delivery of mitochondria to the vacuole. Scoring cells with red, but not green fluorescent vacuoles can be used as a measure of mitophagic activity in cells5,10-12.

A Fluorescence Microscopy Assay for Monitoring Mitophagy in the Yeast Saccharomyces cerevisiae

A robust approach to monitor the delivery of organelles to the acidic lumen of the yeast vacuole for degradation and recycling is described. The method relies on the specific labeling of target organelles with a genetically encoded dual-emission fluorescence pH-biosensor, and visualization of individual cells using fluorescence microscopy.

खमीर में एक निगरानी Mitophagy के लिए प्रतिदीप्ति माइक्रोस्कोपी परख Saccharomyces cerevisiae

Autophagy is important for turnover of cellular components under a range of different conditions. It serves an essential homeostatic function as well as a ...

High-throughput Yeast Plasmid Overexpression Screen

The budding yeast, Saccharomyces cerevisiae, is a powerful model system for defining fundamental mechanisms of many important cellular processes, including those with direct relevance to human disease. Because of its short generation time and well-characterized genome, a major experimental advantage of the yeast model system is the ability to perform genetic screens to identify genes and pathways that are involved in a given process. Over the last thirty years such genetic screens have been used to elucidate the cell cycle, secretory pathway, and many more highly conserved aspects of eukaryotic cell biology 1-5. In the last few years, several genomewide libraries of yeast strains and plasmids have been generated 6-10. These collections now allow for the systematic interrogation of gene function using gain- and loss-of-function approaches 11-16. Here we provide a detailed protocol for the use of a high-throughput yeast transformation protocol with a liquid handling robot to perform a plasmid overexpression screen, using an arrayed library of 5,500 yeast plasmids. We have been using these screens to identify genetic modifiers of toxicity associated with the accumulation of aggregation-prone human neurodegenerative disease proteins. The methods presented here are readily adaptable to the study of other cellular phenotypes of interest.

Here we describe a plasmid overexpression screen in Saccharomyces cerevisiae, using an arrayed plasmid library and a high-throughput yeast transformation protocol with a liquid handling robot.

उच्च throughput खमीर प्लाज्मिड Overexpression स्क्रीन

The budding yeast, Saccharomyces cerevisiae, is a powerful model system for defining fundamental mechanisms of many important cellular processes, ...

Competitive Genomic Screens of Barcoded Yeast Libraries

By virtue of advances in next generation sequencing technologies, we have access to new genome sequences almost daily. The tempo of these advances is accelerating, promising greater depth and breadth. In light of these extraordinary advances, the need for fast, parallel methods to define gene function becomes ever more important. Collections of genome-wide deletion mutants in yeasts and E. coli have served as workhorses for functional characterization of gene function, but this approach is not scalable, current gene-deletion approaches require each of the thousands of genes that comprise a genome to be deleted and verified. Only after this work is complete can we pursue high-throughput phenotyping. Over the past decade, our laboratory has refined a portfolio of competitive, miniaturized, high-throughput genome-wide assays that can be performed in parallel. This parallelization is possible because of the inclusion of DNA 'tags', or 'barcodes,' into each mutant, with the barcode serving as a proxy for the mutation and one can measure the barcode abundance to assess mutant fitness. In this study, we seek to fill the gap between DNA sequence and barcoded mutant collections. To accomplish this we introduce a combined transposon disruption-barcoding approach that opens up parallel barcode assays to newly sequenced, but poorly characterized microbes. To illustrate this approach we present a new Candida albicans barcoded disruption collection and describe how both microarray-based and next generation sequencing-based platforms can be used to collect 10,000 - 1,000,000 gene-gene and drug-gene interactions in a single experiment.

We have developed comprehensive, unbiased genome-wide screens to understand gene-drug and gene-environment interactions. Methods for screening these mutant collections are presented.

Barcoded खमीर पुस्तकालय के प्रतियोगी जीनोमिक स्क्रीन

By virtue of advances in next generation sequencing technologies, we have access to new genome sequences almost daily.  The tempo of these advances is ...

Quantitative Live Cell Fluorescence-microscopy Analysis of Fission Yeast

Several microscopy techniques are available today that can detect a specific protein within the cell. During the last decade live cell imaging using fluorochromes like Green Fluorescent Protein (GFP) directly attached to the protein of interest has become increasingly popular 1. Using GFP and similar fluorochromes the subcellular localisations and movements of proteins can be detected in a fluorescent microscope. Moreover, also the subnuclear localisation of a certain region of a chromosome can be studied using this technique. GFP is fused to the Lac Repressor protein (LacR) and ectopically expressed in the cell where tandem repeats of the lacO sequence has been inserted into the region of interest on the chromosome2. The LacR-GFP will bind to the lacO repeats and that area of the genome will be visible as a green dot in the fluorescence microscope. Yeast is especially suited for this type of manipulation since homologous recombination is very efficient and thereby enables targeted integration of the lacO repeats and engineered fusion proteins with GFP 3. Here we describe a quantitative method for live cell analysis of fission yeast. Additional protocols for live cell analysis of fission yeast can be found, for example on how to make a movie of the meiotic chromosomal behaviour 4. In this particular experiment we focus on subnuclear organisation and how it is affected during gene induction. We have labelled a gene cluster, named Chr1, by the introduction of lacO binding sites in the vicinity of the genes. The gene cluster is enriched for genes that are induced early during nitrogen starvation of fission yeast 5. In the strain the nuclear membrane (NM) is labelled by the attachment of mCherry to the NM protein Cut11 giving rise to a red fluorescent signal. The Spindle Pole body (SPB) compound Sid4 is fused to Red Fluorescent Protein (Sid4-mRFP) 6. In vegetatively growing yeast cells the centromeres are always attached to the SPB that is embedded in the NM 7. The SPB is identified as a large round structure in the NM. By imaging before and 20 minutes after depletion of the nitrogen source we can determine the distance between the gene cluster (GFP) and the NM/SPB. The mean or median distances before and after nitrogen depletion are compared and we can thus quantify whether or not there is a shift in subcellular localisation of the gene cluster after nitrogen depletion.

The fission yeast, Schizosaccharomyces pombe, is a good model system to study basic cellular processes. Here we describe a method to perform quantitative live cell analysis of fission yeast. In this particular experiment we focus on organisation of the genome within the cell nucleus, but the method can also be used to study cytosolic factors.

विखंडन खमीर के मात्रात्मक लाइव सेल विश्लेषण प्रतिदीप्ति माइक्रोस्कोपी

Several microscopy techniques are available today that can detect a specific protein within the cell. During the last decade live cell imaging using ...

4D Imaging of Protein Aggregation in Live Cells

One of the key tasks of any living cell is maintaining the proper folding of newly synthesized proteins in the face of ever-changing environmental conditions and an intracellular environment that is tightly packed, sticky, and hazardous to protein stability1. The ability to dynamically balance protein production, folding and degradation demands highly-specialized quality control machinery, whose absolute necessity is observed best when it malfunctions. Diseases such as ALS, Alzheimer's, Parkinson's, and certain forms of Cystic Fibrosis have a direct link to protein folding quality control components2, and therefore future therapeutic development requires a basic understanding of underlying processes. Our experimental challenge is to understand how cells integrate damage signals and mount responses that are tailored to diverse circumstances.
The primary reason why protein misfolding represents an existential threat to the cell is the propensity of incorrectly folded proteins to aggregate, thus causing a global perturbation of the crowded and delicate intracellular folding environment1. The folding health, or "proteostasis," of the cellular proteome is maintained, even under the duress of aging, stress and oxidative damage, by the coordinated action of different mechanistic units in an elaborate quality control system3,4. A specialized machinery of molecular chaperones can bind non-native polypeptides and promote their folding into the native state1, target them for degradation by the ubiquitin-proteasome system5, or direct them to protective aggregation inclusions6-9.
In eukaryotes, the cytosolic aggregation quality control load is partitioned between two compartments8-10: the juxtanuclear quality control compartment (JUNQ) and the insoluble protein deposit (IPOD) (Figure 1 - model). Proteins that are ubiquitinated by the protein folding quality control machinery are delivered to the JUNQ, where they are processed for degradation by the proteasome. Misfolded proteins that are not ubiquitinated are diverted to the IPOD, where they are actively aggregated in a protective compartment.
Up until this point, the methodological paradigm of live-cell fluorescence microscopy has largely been to label proteins and track their locations in the cell at specific time-points and usually in two dimensions. As new technologies have begun to grant experimenters unprecedented access to the submicron scale in living cells, the dynamic architecture of the cytosol has come into view as a challenging new frontier for experimental characterization. We present a method for rapidly monitoring the 3D spatial distributions of multiple fluorescently labeled proteins in the yeast cytosol over time. 3D timelapse (4D imaging) is not merely a technical challenge; rather, it also facilitates a dramatic shift in the conceptual framework used to analyze cellular structure.
We utilize a cytosolic folding sensor protein in live yeast to visualize distinct fates for misfolded proteins in cellular aggregation quality control, using rapid 4D fluorescent imaging. The temperature sensitive mutant of the Ubc9 protein10-12 (Ubc9ts) is extremely effective both as a sensor of cellular proteostasis, and a physiological model for tracking aggregation quality control. As with most ts proteins, Ubc9ts is fully folded and functional at permissive temperatures due to active cellular chaperones. Above 30 &deg;C, or when the cell faces misfolding stress, Ubc9ts misfolds and follows the fate of a native globular protein that has been misfolded due to mutation, heat denaturation, or oxidative damage. By fusing it to GFP or other fluorophores, it can be tracked in 3D as it forms Stress Foci, or is directed to JUNQ or IPOD.

Cellular viability depends on timely and efficient management of protein misfolding. Here we describe a method for visualizing the different potential fates of a misfolded protein: refolding, degradation, or sequestration in inclusions. We demonstrate the use of a folding sensor, Ubc9ts, for monitoring proteostasis and aggregation quality control in live cells using 4D microscopy.

4D जीवित कोशिकाओं में प्रोटीन एकत्रीकरण की इमेजिंग

One of the key tasks of any living cell is maintaining the proper folding of newly synthesized proteins in the face of ever-changing environmental ...

Analyzing Craniofacial Morphogenesis in Zebrafish Using 4D Confocal Microscopy

Time-lapse imaging is a technique that allows for the direct observation of the process of morphogenesis, or the generation of shape. Due to their optical clarity and amenability to genetic manipulation, the zebrafish embryo has become a popular model organism with which to perform time-lapse analysis of morphogenesis in living embryos. Confocal imaging of a live zebrafish embryo requires that a tissue of interest is persistently labeled with a fluorescent marker, such as a transgene or injected dye. The process demands that the embryo is anesthetized and held in place in such a way that healthy development proceeds normally. Parameters for imaging must be set to account for three-dimensional growth and to balance the demands of resolving individual cells while getting quick snapshots of development. Our results demonstrate the ability to perform long-term in vivo imaging of fluorescence-labeled zebrafish embryos and to detect varied tissue behaviors in the cranial neural crest that cause craniofacial abnormalities. Developmental delays caused by anesthesia and mounting are minimal, and embryos are unharmed by the process. Time-lapse imaged embryos can be returned to liquid medium and subsequently imaged or fixed at later points in development. With an increasing abundance of transgenic zebrafish lines and well-characterized fate mapping and transplantation techniques, imaging any desired tissue is possible. As such, time-lapse in vivo imaging combines powerfully with zebrafish genetic methods, including analyses of mutant and microinjected embryos.

Time-lapse confocal imaging is a powerful technique useful for characterizing embryonic development. Here, we describe the methodology and characterize craniofacial morphogenesis in wild-type, as well as pdgfra, smad5, and smo mutant embryos.

4D confocal माइक्रोस्कोपी का उपयोग Zebrafish में Craniofacial Morphogenesis का विश्लेषण करना

Time-lapse imaging is a technique that allows for the direct observation of the process of morphogenesis, or the generation of shape. Due to their optical ...

Microscopy of Fission Yeast Sexual Lifecycle

The fission yeast Schizosaccharomyces pombe has been an invaluable model system in studying the regulation of the mitotic cell cycle progression, the mechanics of cell division and cell polarity. Furthermore, classical experiments on its sexual reproduction have yielded results pivotal to current understanding of DNA recombination and meiosis. More recent analysis of fission yeast mating has raised interesting questions on extrinsic stimuli response mechanisms, polarized cell growth and cell-cell fusion. To study these topics in detail we have developed a simple protocol for microscopy of the entire sexual lifecycle. The method described here is easily adjusted to study specific mating stages. Briefly, after being grown to exponential phase in a nitrogen-rich medium, cell cultures are shifted to a nitrogen-deprived medium for periods of time suited to the stage of the sexual lifecycle that will be explored. Cells are then mounted on custom, easily built agarose pad chambers for imaging. This approach allows cells to be monitored from the onset of mating to the final formation of spores.

We provide a reproducible basic method for the long-term microscopy of the fission yeast sexual lifecycle. With minor adjustments described, the presented protocol allows research focus on different steps of the reproductive process.

विखंडन खमीर यौन जीवन चक्र के माइक्रोस्कोपी

The fission yeast Schizosaccharomyces pombe has been an invaluable model system in studying the regulation of the mitotic cell cycle progression, the ...