C2006/F2402 '14 OUTLINE OF LECTURE #12

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1 C2006/F2402 '14 OUTLINE OF LECTURE #12 (c) 2014 Dr. Deborah Mowshowitz, Columbia University, New York, NY. Last update 03/04/ :24 PM Handouts: 12-A -- mrna processing 12-B -- Alternative processing of mrna 12-C -- Examples of Translational Regulation PPts shown at start of class ("How many people are dead?") are posted on Courseworks. Correction of terminology in section IV-B was made after morning lecture -- changes are marked in blue. I. Overall Regulation of Eukaryotic Gene Expression -- What has to be done to make more or less of a protein? A different protein? What steps can be regulated? A. If cells make different proteins, how is that controlled? If two eukaryotic cells (from the same multicellular organism) make different proteins, what is (usually) different between them? Examples: Chicken oviduct cells make ovalbumin -- chicken RBC make globin* Human liver cells make transferrin -- human precursors to RBC make globin *Note: Chicken RBC, unlike human RBC, have nuclei The Question: What is different in the two types of chicken cells? Or the two types of human cells? 1. Is DNA different? (No, except in cells of immune system & gametes.) 2. Is state of chromatin different? (Yes -- see experiment described on RP 5 or Becker (23-17).) 3. Is mrna different? (Yes). A consequence -- cdna libraries. cdna = complementary DNA = DNA made in vitro by enzymes (including reverse transcriptase), from an mrna template. Since mrna is different in different tissues, you can get tissue-specific sequences from a cdna library. (cdna library = collection of all cdna's from a particular cell type.) DNA from each cell type is the same; mrna and therefore cdna is not. See Becker fig (23-20). For a problem about DNA & cdna libraries, see 14A Why is the mrna different? a. Transcription is usually different. See notes of last class. Only selected genes are transcribed in each cell type, and RNA's from those genes are processed to make mrna. (For an experiment that shows this, see figure (23-19) in Becker.) b. Processing can be different: Splicing and processing of the same primary transcripts can be different (in different cells or at different times). Different mrna's (& therefore proteins) can be produced from the same transcript by alternative splicing and/or poly A addition. Details & example below and on handouts 12-A & 12-B). B. How can amount of protein synthesized be controlled? If cell makes more or less protein, which step(s) are regulated? 1. In prokaryote (for comparison) -- process relatively simple.

2 a. Most regulation at transcription. b. Translation in same compartment as transcription; translation follows automatically. c. Most mrna has short half-life. 2. In eukaryote -- Gene expression has many more steps & complications than in prokaryotes -- more additional points of regulation -- not just at transcription. See Becker fig (23-11) or Sadava fig (16.13). a. Transcription is main point of control, but other steps are often regulated too. b. Transcription & translation occur in separate compartments. Translation does not follow automatically. (1). 2. Transcript must be processed (capped, spliced, polyadenylated, etc.) -- any of these steps can be regulated, and there is more than one way to process most primary transcripts. (Example below.) (2). mrna must be transported to cytoplasm. (3). Translation can be regulated (independently of transcription) -- can control usage and/or fate of mrna, not just supply of mrna. For any particular mrna, can regulate 1 or both of following: (a). Rate of initiation -- can control how often ribosomes attach and start translation. (b). Rate of degradation -- can control half life of mrna. c. Different eukaryotic mrnas have different half-lives. Some mrna's are long-lived and some have a very short half life. d. Protein must reach its proper destination (nucleus, mitochondria, ER, etc.) -- how this works was covered in previous lectures. C. Once protein is made, how is protein activity regulated? There are multiple modes of Post-Translational Regulation. Details below. II. Processing of Eukaryotic mrna transcripts Once transcription gets started, what does it take to get a functioning eukaryotic mrna? All necessary details are included here and on handout, but splicing was discussed last term and will be covered only briefly in class. A. Caps and poly A -- See handout 12A. Most eukaryotic transcripts that will be used as mrna must be modified on both ends (as well as spliced) before they can be transported to the cytoplasm and used for translation. A "cap" is usually added to the 5' end and a "poly A tail" to the 3' end. See Sadava 14.9 (14.10). The steps involved are shown on handout 12A. (Numbers below match steps on handout.) 1 Beginning of transcription. a. Start: The start of transcription is usually indicated by a bent arrow. b. Symbols: The boxed areas of the DNA = exons; plain DNA between them = intron.

3 2. Capping. a. What's a cap? A modified G is added to the 5' end of the transcript shortly after transcription begins, while the transcript is still being made. b. How is cap added? The G is added "backwards" so there is a 5' to 5' connection. (For the curious: The structure of the cap and how it is connected to the transcript is shown in your texts; see fig. Becker fig (21-18.) c. Symbols: The cap is represented on the handout as a filled circle. 3 Transcription continues to or slightly beyond the end of the gene or transcription unit. a. A fixed stop? There may be no fixed stop for transcription in eukaryotes (for production of most mrna); the addition of poly A (see below) may determine the exact 3' end of the transcript. b. Poly A: Most but not all eukaryote mrna's contain poly A. c. Reminder: in eukaryotes production of rrna & trna are carried out by different RNA polymerases which have somewhat different properties. these RNA's do not have poly A. (For details see texts.) 4 & 5. Polyadenylation. See Becker fig (21-19). a. What's a polya tail? A poly A tail -- a string of A's a few hundred long -- is added to the 3' end of the RNA. b. Growth of polya tail: Growth is 5' to 3' using ATP, enzyme, and splitting off pyrophosphate as usual. No template is used. c. Addition Sequence: The sequence AAUAAA is the signal for the appropriate enzyme to cut the transcript a bit downstream and add the string of A's. (Downstream = in the 3' direction on the mrna or sense strand.) d. What's not encoded in the DNA? The A's on the 3' end and the G of the cap are not encoded in the template DNA. e. Timing: On the handout cleavage of transcript = step 4; addition of poly A = step 5. These two steps may occur simultaneously.

4 f. There may be more than one possible site for addition of poly A. Therefore the 3' end of mrna can vary. An example is considered below. 6. Set up for Splicing. Nothing has happened to the RNA in step 6 except that it has been labeled to indicate exons and introns (so we can explain splicing). a. Timing: By the time the transcript is released from the DNA it already has a cap on the 5' end and a poly A tail on the 3' end. This RNA -- modified on both ends but not spliced -- is usually called the primary transcript or pre-mrna. See Becker fig (21-22). b. Terminology: Some texts refer to unmodified RNA as the primary transcript, but such a state doesn't really exist, since the pre-mrna is modified before it is released from the DNA. c. The RNA is now ready for splicing (steps 7-9 on handout). Note: Splicing may begin prior to polya addition; see below. B. Splicing of Eukaryotic mrna -- Review from last term (not all details will be covered in class) 1. A typical picture of a gene with introns and exons (for reference). The picture below shows a section of the sense strand of the DNA that includes a gene with 3 exons and 2 introns. (The picture on the handout has 2 exons and one intron.) Conventions: The picture on the handout shows double stranded DNA, but genes are often shown as in the picture below, with only the sense strand actually drawn in. Transcription would start at the 5' (left) end of exon 1 and go to the right. Important features of intron: Branch point, 5' splice site (also called the donor site) and 3' splice site (also called acceptor site). These are shown for the first intron only. See also fig (21-22) in Becker or Sadava fig (14.11). Terminology: "donor and acceptor site" describe splicing from the exon's point of view; "5' and 3' splice site" describe it from the intron's point of view. Also note that the region to the left of exon 1 is NOT an intron -- it is not part of the gene. It is part of a spacer in between this gene and the previous one. 2. Splicing Details -- See bottom of handout 12A a. General Features (1). Splicing out of each intron occurs in 3 steps (see handout, steps 7-9). At each step the

5 parts of the transcript are held in place by the spliceosome. The steps are repeated for splicing of each intron -- many RNA's have many introns. Details are below. (2). Terminology The splice junction at the 5' end of an intron is called the 5' or donor site; the splice junction at the 3' end of an intron is called the 3' or acceptor site. b. Steps of splicing. See handout 12A at bottom. See also Becker fig (21-24) or Sadava (14.11). All the steps are catalyzed by the spliceosome, as follows: (1) Step 7 -- RNA transcript forms loop for removal of intron. (2). Step 8 -- Cut at 5' end of intron (a). 5' splice site (donor site) is cleaved (b). loose end of intron (5' end of intron) attaches to branch point in the middle of the intron, forming lariat-shaped structure. (3). Step 9 -- joining of exons (a). The 5' donor site attaches to the 3' acceptor site, joining the two exons and releasing the intron in the form of lariat. (b). The lariat will be degraded and the nucleotides will be recycled. (c). The RNA containing the exons (without the introns) will be transported to the cytoplasm and translated. c. N.B: Prokaryotes do not have introns and lack the machinery needed to remove them. 3. Do exons and translated regions coincide? See diagram at bottom of 12A. Review from last term: a. Exons = sections of genes that are represented in the mrna. Exons include untranslated 5' and 3' regions as well as the translated regions. Exons and amino acid coding regions do not coincide, because there are extra untranslated sections in the mrna. Exons and mrna regions do coincide. b. Exons are not = protein coding sequences, as some texts imply. (The diagram in Sadava fig (14.7) is incorrect.) Exons include protein coding sequences, but also include sequences (UTRs) that are represented in the mrna but do not code for amino acids. (The Sadava diagrams have no UTRs.) c. Where are the UTRs? (1). Leaders. At the 5' end of the mrna, there is a 5' untranslated region (UTR) or leader before translation begins (before the first AUG). The DNA coding for this region is transcribed, and the RNA is not spliced out, but this region of the mrna is not translated. The 5' UTR is encoded in one or more exons. (2). Trailers. At the 3' end of the mrna, there is a 3' UTR or trailer that is after the stop codon. The DNA coding for this region is transcribed, and the RNA is not spliced out, but this region of the mrna is not translated. The 3'UTR is encoded in one or more exons.

6 III. Regulation at Splicing -- Results of Alternative Processing A. There are two ways to get a collection of similar proteins 1. Gene families -- multiple, similar genes exist due to duplication and divergence of genes. Example: the globin genes constitute a family. Different family members code for myoglobin, beta-chains, alpha-chains, delta-chains, etc. Other gene families include the GLUT, SGLT, and IF (intermediate fillament) families. 2. Alternative splicing or processing (See below) -- only one gene, but primary transcript spliced in more than one way. Examples: fibronectin, soluble and membrane bound antibodies. B. The Genome vs the Proteome -- You can get many different mrnas from a single gene by the processes listed below. Therefore the number of possible proteins (the proteome) greatly exceeds the number of possible genes (the genome). Processes that yield different mrnas: 1. Starting transcription at different points 2. Ending transcription (adding poly A) at different points 3. Splicing out different sections of the primary transcript -- alternative splicing. See Becker fig (21-25). What is considered an 'intron' or 'exon' may vary, depending on the way the primary transcript is spliced. C. An example of alternative processing -- Production of antibody (immunogloblin) in B cells. See handout 12B and Becker fig (21-31) -- how to get either soluble or membrane-bound antibody from alternative processing of the same transcript. (See Sadava fig for another example.) 1. Antibody can be membrane bound or secreted. Fate of antibody depends on whether peptide has a hydrophobic sequence near one end or not. Hydrophobic sequence can anchor the protein in the membrane -- becomes a transmembrane (TM) sequence. a. If Ab has a potential TM sequence: Hydrophobic section locks into membrane of ER as protein is made. Vesicle buds off ER and protein travels through cell as part of vesicle. Protein remains in membrane of vesicle. When vesicle fuses with plasma membrane, Ab stays in membrane. b. If Ab has no TM: Ab enters lumen of ER as protein is made. Vesicle buds off ER, and protein ends up in lumen of vesicle. When vesicle fuses with plasma membrane, Ab is secreted. 2. Gene has two alternative polya addition sites. Which one is used determines final location of protein. a. Option 1: If poly A addition site #1 (at start of 'intron 4') is used, protein contains no hydrophobic potential TM sequence, and protein is secreted. (Note: 'intron 4' is spliced out in option 2, but the beginning of 'intron 4' is included in the mrna in option 1.) b. Option 2: If the other poly A addition site (at end of exon 6) is used, protein contains hydrophobic sequence encoded by exons 5 & 6, which becomes a TM sequence, and protein stays in plasma membrane. c. Terminology: Poly A addition site #1 is usually considered to be in an intron since it can be spliced out (in option 2). Alternatively, it can be considered an extension of exon #4 (in option 1).

7 3. mrna can be spliced and/or poly A added in two alternate ways. Location of protein (antibody) depends on whether splicing of intron 4 or poly A addition happens first. Both processes (splicing and polya addition) occur concurrently. Either a. Poly A adding enzymes get there before the spliceosome. In that case, poly A is added to site #1 near end of exon 4, and rest of intron 4 (and rest of gene) is never transcribed, or b. The spliceosome gets there first. In that case, Intron 4 is transcribed and spliced out before poly A can be added. (In this case, poly A is added at the end of exon 6 instead.) 4. Why are 2 forms of antibody needed? a. Membrane-bound form of antibody: Serves as receptor for antigen = trap to detect when antigen is present. Binding of antigen (ligand) to antibody (receptor) serves as trigger to start secreting antibody. b. Secreted (soluble) form: Acts as effector -- carries out major function of immune system - - binds to soluble antigen in body fluids and triggers destruction of antigen in multiple ways. To review regulation & alternative splicing, try problems 4-13 & IV. Regulation at translation. A. How to control rate of translation? In principle: 1. Can regulate half life of mrna (control rate of degradation). a. In prokaryotes most mrna's have a short 1/2 life; in eukaryotes this is not necessarily so. b. Different eukaryotic mrna's have very different half lives. 2. Can regulate rate of initiation of translation (control how effectively translation starts). B. Some Famous Examples of Regulation of Translation. (The principles are more important than the details, but diagrams are on handout 12C to make note taking easier.) 1. Use of a regulatory protein: -- Have a protein that binds to mrna (or some other part of the translation apparatus) and affects either initiation and/or degradation, depending on where it binds. Two examples: a. Regulation of synthesis of Ferritin & Transferrin Receptor (& intracellular iron levels). Function: Ferritin is an intracellular protein that stores excess iron. (Transferrin & its receptor were discussed in the section on RME.) Overall: Regulatory system is similar to induction/repression, but it is translation, not transcription, that is affected by the regulatory protein. Details of Role of Regulatory protein: (1). Protein acts like a (prokaryotic) repressor, but binds to regulatory sequence in mrna, not DNA. (2). Regulatory protein is allosteric, and level of small molecule effector (Fe) inactivates the regulatory protein.

8 (3). The regulatory protein binds to mrna in the absence of Fe, not when Fe is high. (4). Active form of repressor protein binds to more than one mrna. Binds to mrna for ferritin and to mrna for transferrin receptor. (Blocks initiation of translation of one mrna and degradation of the other.)* This is another example of coordinate control. There is one trans-acting factor here (regulatory protein), but both mrna's have the same cis acting sequence. See Becker, figs & (23-33 & 23-34) if you are curious about the details. *A question to think about: Regulatory protein binds to mrna for protein B at 5' end (blocking initiation) and to mrna for protein A at 3' end (blocking degradation), as shown on handout 12C. Given the information above, which is protein A, and which is protein B? Which one is ferritin and which one is the transferrin receptor? You can check your answer in Becker or using this diagram. b. Regulation of globin synthesis by heme -- Handout 12C. (Becker fig in 7th ed only). Heme (the prosthetic group of hemoglobin) stimulates synthesis of globin (the protein part of hemoglobin). In this case, heme prevents inhibition of translation. In the absence of heme, inhibition occurs, and translation is blocked. No globin produced. Heme blocks the inhibition. Therefore, in the presence of heme translation proceeds. Heme relieves the block in translation, and globin is made. Interesting features of this case worth noting are: (1). Inhibition of inhibition results in stimulation; in other words, (-) X (-) = (+). (2). Another example of coordinate control. This system ensures coordination between the supply of heme and of globin. Globin is useless without heme. (3). This is an example of modifying protein activity by reversible, covalent modification. The protein that blocks translation in this case is reversibly phosphorylated. (Other proteins needed for translation are also regulated by phosphorylation.) FYI: Heme works by interfering with phosphorylation -- it blocks a kinase from phosphorylating a critical translation factor (elf2 =eukaryotic initiation factor 2). Phosphorylation of elf2 (in the absence of heme) inhibits elf2 and blocks translation. This is another example of a protein (elf2) that has active and inactive forms, and phosphorylation (or dephosphorylation) interconverts the two forms. 2. Use of a regulatory RNA -- RNA interference (RNAi) a. Trans acting factors can be RNA. Not all regulatory factors are protein -- some are short RNA's. (These are usually derived from double stranded RNA -- See Becker figs & (23-35 & ) b. How does a short RNA affect translation? (1). Inhibition (usual case): Small RNA binds to mrna Formation of double stranded RNA. This triggers degradation &/or inhibition of translation of the mrna.

9 (2). Stimulation: Some recent cases have been discovered in which small RNA binds to mrna and 'up regulates' translation. Mechanism so far unknown. c. Use in Regulation: Cells naturally produce micro-rna's that bind to mrna's and regulate translation as above. The use of short regulatory RNA's to block translation appears to be important during regulation of development. See Becker fig (23-36). d. Use in the Lab as a tool: Called RNAi = RNA interference. The use of artificially added short double stranded (ds) RNA to block transcription*/translation and turn genes off is very common. (See Becker fig [23-35].) Enzymes of cell convert added ds RNA into short single stranded RNA that interferes with translation and/or transcription* as in b. Same effect as adding antisense RNA (but works better). Fire & Mello received the 2006 Nobel prize in Physiology or Medicine for discovering RNAi. *We have concentrated on effects of RNAi on translation. However, some short RNAs may inhibit transcription by affecting the state of chromatin -- they could stimulate methylation of the histones and/or DNA. V. Post Translational Regulation. Don't forget: regulation occurs after translation too -- after proteins are made, their activity can be modulated, as for EIF2 above. Many examples of post translational modification have already come up and more will be discussed later. Here is a summary (mostly review): A. Covalent Modification. Proteins can be modified covalently either reversibly or permanently. Some examples: 1. reversibly -- by phosphorylation and dephosphorylation; acetylation & deacetylation, etc. 2. Irreversibly -- by removal of N-terminal met., addition of sugars -- glycosylation, etc. See problem 6-3. B. Noncovalent Modification. Proteins can be activated or inhibited by reversible noncovalent binding of other factors -- small molecule allosteric effectors, other proteins such as calmodulin (an important Ca 2+ binding protein to be discussed later), etc. C. Degradation. Proteins can be selectively destroyed or 'turned over'. 1. Half Lives Vary. Not all proteins have the same half life. 2. Significance: Important example of a family of proteins that all have a short half life = cyclins; control progression through cell cycle. Different cyclins control transitions from G1 to S, G2 to M etc. Cyclins are made as needed and degraded immediately after use. 3. mrna vs Protein: The term 'half life' can refer to the stability of the mrna or the stability of the protein. Both mrnas & proteins can have short or long half lives. For cyclins, both the mrnas for the proteins and the proteins themselves (the cyclins) are degraded after use. More on this when we cover the details of the cell cycle. 4. Role of Proteasomes: Most cellular proteins to be degraded are tagged with multiple molecules of ubiquitin and broken up in proteasomes. (Becker, fig or Sadava fig (16.24) ). See notes of lecture 8 of for more details on proteasomes. D. Location. Proteins can activated or inhibited by a change of location. For example, transporters like GLUT4 only work if positioned in the plasma membrane; if they are sequestered in vesicles they are inactive. Transport of glucose

10 into the cell can be regulated by moving the GLUT4 in and out of the membrane. IV. Introduction to Signaling (Chap. 7 of Sadava, Chap. 14 of Becker. Detailed references next time.) A. Big Issues 1. What does signaling involve? a. How are messages sent from one cell to another? b. How are signals received? c. How do signals produce a response in the target cell? 2. How does signal transduction occur? How does a signal from outside produce an response inside the target cell? a. How are signals transmitted across membranes? b. How is amplification of the signal achieved? 3. Why bother with signaling? What is it for? a. It's needed so events in a multicellular organism can be coordinated. b. It's not enough to regulate what one cell does! B. Usual Method -- one cell secretes signal molecules that bind to a receptor on (or inside) a target cell amplification big effect in target cell. Types of amplification: 1. Opening ion channels -- opening a few (ligand gated channels) triggers opening of more (voltage gated channels), which causes a big change in ion concentrations and protein activity. 2. Cascades of modifications -- for example, adding phosphates to enzymes that are kinases or phosphatases, activating them, so they modify more proteins, and so on. 3. Affecting transcription &/or translation -- make more of target protein. C. How to Classify Signal molecules 1. By type of cell that makes them and/or target location. Where do the signals come from, and where do they go? (endocrine, paracrine, etc. -- handout on this next time.) 2. By chemical properties -- hydrophobic (lipid soluble) or hydrophilic (water soluble)? Next Time: Signaling Details: Signals, Receptors, Modes of Amplification & Transduction