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BIOL 2321_Microbiology for Science Majors - 2321_MW4_2_14_23_Lecture
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00:04 Mhm. Yeah. Alright. So happy valentine's day. Okay. Um
00:30 so we're gonna wrap up Chapter five . Okay. Uh so obviously that
00:40 um today is the end of you . So we started to on thursday
00:51 would be a viruses part one. as a flipped class. So recorded
00:58 for that has been up since last . So um but nothing on Thursdays
01:04 example, unit two is all exam stuff. Okay, so uh somebody
01:11 smart work due tomorrow. Okay, not a long one, but I
01:19 remember that that's due tomorrow. So of course exam on later this
01:25 Uh You have any last minute you know, I'll email or office
01:31 , you know whatever works and I think any, I don't think I
01:39 anything else. Uh So let me let's just begin with kind of a
01:46 Of last time. Okay, so finished up chapter four with bathroom information
02:00 in the school information. So I uh both those things are can certainly
02:07 awful information, nutrients driven, you , you have to have influx of
02:12 to maintain that large fire film. In fact even initiated. Um remember
02:19 were all about a surface and Right? Um The formation occurs under
02:30 deprivation but of course other things as , uh any kind of distress situation
02:36 potentially induce in those information. Um of course is a very uh resistant
02:44 . Okay and um uh so then went into chapter I talk about zero
02:54 . So in a nutshell basically Couple things. So one living in an
03:03 world, auction being very reactive can with molecules creating these reactive types super
03:16 , etcetera. And though they interact proteins and fake acids, other molecules
03:24 them. And so any organisms living the presence of air, whether they
03:31 02 or not, okay. If going to survive in that environment,
03:35 need to have protection. Right? have ourselves had the same thing,
03:40 have protection against it. We have . O. D. We have
03:44 a lace and proxies in ourselves to us with that. Okay. And
03:48 similarly, other microbes that live in 02 have that protection. So that's
03:58 is uh do they use oxygen? . And what's the requirement?
04:05 So some some must have it at concentrations. Others can't handle that because
04:13 don't have the full complement enzymes or have lesser amounts of them,
04:18 Right? But they still need to they can only handle it at lower
04:23 . So you're Arabs clarifies um Faculty Arabs can live with or without
04:30 They can they can do the full of respiration, aerobic anaerobic and
04:37 Right. And so it all depends what situation they're just they're present.
04:42 not What's the best thing? And they of course have the protection
04:47 they can live you know in in in an auction environment. And then
04:51 the middle is kind of the But in the middle of this diagram
04:57 anna robes. Right? So and a rope can be does not use
05:04 by definition as part of their They ferment or anaerobic respiration. Um
05:10 the what differentiates the an arrow and arrow tolerant. Arab is the presence
05:17 protective enzymes. The does not have . So it cannot live in 02
05:25 . Has to be away from Okay, um serotonin and Rokan.
05:31 it doesn't use up too. But has the protection so it can live
05:35 their environment. Yeah, it's basically distinction between these things. Right.
05:41 so biofilm and of course any questions that. Okay, so then we
05:50 right into the last half of five is basically focused on death if you
05:55 . Okay. Death of microbes. . And so of course we're targeting
06:00 you apply any kind of antimicrobial You're gonna reduce levels of all
06:05 But of course the ones of interest those that are pathogens because they can
06:09 disease. Right. So um and there were focused obviously on the right
06:16 of that batch growth curve. Death right? Occurs exponentially. And
06:22 it's about how can we uh add to kill microbes that will do so
06:32 quickly and at a fast rate. , So logs of death is what
06:36 into them. Okay. And so looked at these four terms. This
06:40 where we ended last time. All , so sterilization and exceptions disinfection.
06:47 , So we know um sterilization that you sterilized, there were no
06:54 spores, viruses gone. Okay. not 99.9% killing it's 100%.
07:02 And so of course disinfection interceptions, don't do that to reduce numbers.
07:09 still remember the Subsys on tissues, tissues. Disinfection of is on inanimate
07:18 . Right? Thus you can have two chemicals. Disinfectant can be much
07:24 . Right, concentrated more harsh if will think bleach versus isopropyl alcohol.
07:31 . Leeches are disinfected as a purple and accepted. So in sanitation relates
07:37 to overall reduction of microbial numbers because represents kind of the level of
07:46 Right? So I always use the of a restaurant kitchen where you try
07:52 minimize the foodborne africa what illness and . And so using gloves,
08:00 uh keeping the area clean, disinfecting , um uh food and proper
08:09 So any of these things are things can potentially lead to a foodborne
08:14 So that's kind of sanitary practices kind what defines or hygienic practices is what
08:21 sanitation. Okay, so that kind nutshell is was last lecture.
08:28 Any questions. Okay, so let's have some more terminology. So here
08:38 so focused on the course production of numbers. So obviously we do that
08:45 affecting their growth right now are either growth or just outright killing them.
08:53 . And so we have these terms static bacterial silo bacterial politic okay to
08:58 that. So anything that's a bacterial agent, like the name implies
09:02 you're not actively killing cells but you're kind of inhibiting their growth.
09:08 And the killing occur, effects occur bacteria seidel and bacterial agents.
09:15 And so if you look at the here. Alright, so let's focus
09:21 the solid line and all of My dad prefers the viable cell
09:27 Okay, so the solid line, there's two measurements going on here.
09:33 a bible cell count which is done briefly explain. You don't need to
09:39 their exam or anything you do in lab. Later on basically you'll have
09:43 sample if you know what the viable count is in there. Right?
09:51 cell count. What you do is have to get these on a
09:59 Okay. In such a way that get isolated colonies, this is not
10:06 a street plate, This is using nothing where you're basically putting a lot
10:13 liquid on top of the plate, you're gonna spread it like a windshield
10:17 right all across the plate. And you you have to dilute it requires
10:26 because you know, a social spread the bacterial, you plop 1/10 of
10:32 meal on a plate as is is gonna be some themselves. And it
10:36 all rode together, there would be big long color. Right? And
10:42 you can't get any distinguishing and then colonies. Right? So how do
10:46 get that? But you have to , right? So you actually carry
10:49 a series of solutions and you sample ones to see which gets you,
10:54 know, lots of isolated colonies in form. Because the premise is that
11:01 colony Equals one cell. Okay, makes sense. You put one little
11:10 on a plate, it's gonna We're almost neighbors will come together to
11:13 a colony visible, but it originates one cell. So that's the
11:18 It's true for the most part, there are exceptions, but for most
11:21 that's true. So what that means you can't call it on the
11:25 You're counting cells that are running that tube, Okay, Because that's where
11:30 came from. Right? So what have to do again, we're not
11:34 into all the details. You there's calculation you do just back calculate based
11:38 the delusion made and it gives you parameter called cells. For me.
11:45 complicated. Right? It's also called a few per meal for colony forming
11:53 . Again, your lab, you'll learn this stuff, but that's how
11:58 get a viable capital because things are on your plate are viable cells,
12:04 ? So what does that tell Well, if we look at this
12:10 growth curves starting from this portion. ? Over here obviously as we measure
12:18 bible cells were going up. it's growing. Okay. Uh here
12:25 the arrows. You see the that's where we're adding our whatever it
12:31 antimicrobial agent. Okay. Of course see at that point different responses.
12:41 , what's going on beyond the Our agent. Okay. So the
12:48 graph you see here plot is the line. Okay. The dash line
12:53 totally count. And I suspect this done with a microscope. You look
12:59 the microscope samples and just look at . There's ways you can count cells
13:04 well. Um but it really doesn't between live and dead. Just all
13:09 can't really tell which one's the dead for alive. Okay. But you
13:14 if it's growing you're seeing an increase the number of cells. Okay.
13:20 we add our agent. What's going on the left side now? Past
13:24 arrow in that interval. So you back to your static agent inhibits
13:31 So you're not gonna see any You don't kill him. If you
13:36 killing going on, you see that count going. So basically you have
13:41 flat no growth. Okay. No but no growth. Okay. No
13:47 growth and the under the microscope, number of cells are basically staying the
13:52 in that period. Okay, so go to both bacterial cyanobacteria, literally
13:58 of those our drops and cell count the agent is actively killing the
14:04 Right? So as you take samples here on this side. Okay are
14:12 less and less colonies on your plate means viable counts going down. Something
14:17 killing the thing. Okay so the then is so that's common to both
14:24 that's what they do. That's your bacteriological agents killed. Right then.
14:28 the difference here with this pattern? that pattern and see what pattern works
14:38 nope. This pattern and that okay the dash line. Um So if
14:49 are in both scenarios death is a and we know that because of the
14:54 why are we seeing the dash Lyons come back to recital and going down
15:00 bacterial lyric anybody. So visualize you're under the microscope. The bible counsels
15:10 you that is going on right But bacteria side bacteria stat sir bacteria seidel
15:18 . Those cells are under a microscope changing a number. They're kind of
15:22 that okay. Are these dead cells yes or not? Absolutely that for
15:38 because that's telling you that This this telling you that dang it.
15:48 Stupid. This is telling you That is telling you that it's going
15:52 . Okay so here two cells are right at the back spine is down
15:59 . So what gives so it's here the metro societal agent but they're
16:07 Right? But the operative word here lice you can kill cells without
16:15 That's what's going on. The Sidelight right? Um They're just they're
16:21 there's not being lice that communicated blows up. Okay detergents very commonly those
16:28 of antimicrobials melt dissolve membranes. So certainly gonna lice itself. So it
16:37 on the back paralytic agent. You really see anything on your microscope after
16:40 period of time. Pretty much right the beginning. Right? And so
16:45 keeps going down down down down they disappear right? Because they're being back
16:51 the spinal agents do it differently. still kill the cells are just cells
16:55 intact so that's what's going on. um Now um so there's so this
17:05 illustrates the same point. Okay so um we just see to history says
17:16 okay so in the bottom you see this would be likely what a looking
17:23 a recital electrostatic bacteria, asylum might something like this. All right after
17:28 added our chemical or biological agents. let's just say this is the point
17:34 the arrow is okay and this is seidel static. Alright So what we're
17:41 under the I'm sorry like bacterial igic here. Okay so the soldier is
17:49 because they're being nothing complicated. Any about that. Yeah bacterial bacterial.
18:01 yes. Typically yes because you can't if you're just doing a complete visual
18:10 all the cells look the same. can't distinguish between live and dead.
18:14 you can um there are fluorescent dyes can use nowadays that actually distinguish between
18:22 and dead cells. So you could nowadays under a microscope you put on
18:27 I think it's called accurate and orange . Live cells so you can actually
18:31 distinguished by color but the cells are there but now you can visualize by
18:36 different types of dyes nowadays. Yeah that that okay. Uh Okay
18:46 um okay let's look at this question . Okay so this gets us in
18:52 next couple of things here which is uh logs of death. And the
18:56 values is kind of the parameter that's to evaluate how well an antimicrobial agents
19:04 . So this is says uh the seniors of course is the definition.
19:10 right here this okay so if this it is added to a culture containing
19:21 of the six cf. You per . And the d value is two
19:26 . How many bible cells are left eight minutes Uh predict 99% correctness,
19:44 . Let me open it up. now you can answer. Okay let's
20:27 down here from 10. Alright so it is going to be d okay
20:44 let's just go through so we start that number of cells, one log
20:49 death every 10 minutes. So we 2468 right down to 65432. Okay
20:58 um and so this parameter of logs death Is used in different ways.
21:08 sometimes it's just it's just one log kind of these kind of products have
21:16 of modified to their particular product. it's not unusual to see 12 logs
21:20 death for some things. So it's kind of depends and so a lot
21:25 factors go into that, you know kind of disinfectant agent it is um
21:33 are they what it meant to Okay so there's different ways manufacturers to
21:38 this but across the board is obviously killing cells and doing so in a
21:44 fashion but they kind of each have own particular um tweak to it.
21:53 Now Okay so the value. So just another way to come up with
21:59 value. So very typically you have culture so this one happens to be
22:04 28. Right then they do the to it. And of course you
22:09 a negative slope, right? Death then you go, Okay let's pick
22:14 values that are a log apart. ? So 10 to the fifth then
22:19 fourth just extrapolate. Okay and you a difference of about a minute.
22:24 I forget what this was. But the value here will be considered one
22:28 , one minute to get one log that. So lots of things affect
22:33 efficacy. Right, so talk about load that refers to what's the self
22:40 of what you're trying to treat. loaded with microbes, is it not
22:46 will require you know it may require treatment in terms of concentration of
22:53 longer time of exposure, these kinds things. Um the exposure time population
23:01 . Is it is it full of uh in those four foreign bacteria?
23:09 . Well that may require something different it was just a cola or
23:13 But to be honest and practical sense don't really get those kinds of analysis
23:18 something you're about to disinfect unless it something where your maybe your treatment is
23:25 not working then you may need to may be required to do that kind
23:29 analysis. But for most things you get to that level where you just
23:33 to find out what exactly do you I'm cleaning and trying to get rid
23:37 ? You don't normally do that for practical standpoint but you know it could
23:41 a difference in some cases. Organic I think is probably particularly important.
23:48 and um using any kind of pretty sure it probably says so on
23:55 Lysol bottle or whatever your favorite is . It will say things surface first
24:01 applying that's because dirt organically basically think dirt that's already on the surface.
24:07 ? So not really including the all this could be part of it
24:11 it's very dirty which are trying to . It's best to clean it
24:16 then disinfected otherwise disaffected may not be too the microbes efficiently. Alright,
24:23 cleaner surface then disinfect uh crossing this the nature of the chemical? Uh
24:31 it very harsh and can maybe harm surface you're trying to clean? Uh
24:36 it how stable is it? Is is it light sensitive? Some things
24:40 light sensitive that don't work as well they're exposed to light? Or is
24:45 is it volatile? Is it like alcohol based disinfectant versus a maybe an
24:52 based um have all basically they evaporate quickly. They may not have a
24:59 power or something like uh we called are more sticky if you're the last
25:06 volatile Ized. But can you leave weird film on your surface?
25:11 you know, all these things have pluses and minuses point is there are
25:15 of things that can affect the efficacy these things. Okay. Um Now
25:23 now you might think there's some not an auto play, right? Will
25:28 everything all at once. Right. you you don't really ever see I've
25:34 seen anything that the treatment that gives that kind of response. Okay.
25:38 they all die it once. Because it can be very fast.
25:42 can be a very fast rate. , But not all at once because
25:47 it's all about any population that you're Okay, a lot of variables go
25:55 it. So think of if it's particularly concentrated with cells, right,
26:01 cells in the periphery likely going to killed more quickly than those that are
26:06 the interior. Right? So that there is going to give you a
26:09 to kill it. But regardless, know, the members of each
26:15 that population are gonna die when they enough damage. Right there, proteins
26:22 proteins have been uh destroyed or the and or gas. And so we
26:29 to a point where it's too I'm dead. That's not gonna be
26:33 the same for every cell in the . That's why there's always a great
26:37 uh granted it could be fast but still gonna be a rate. Um
26:45 questions about that. So uh let's at so I just threw this one
26:51 . I'm not gonna expect you to again this and laugh, but this
26:56 what we call the disc disc diffusion . Okay, and uh this next
27:03 um this diffusion method and I can't with my fingers. Let me take
27:09 off. Try this. Pen is finicky here this oh, there we
27:15 . This diffusion method, right? probably have seen this, I'm
27:20 And the little paper disks. Very contest antibiotics come come like this.
27:26 can test the efficacy of antibiotics but you can take by these paper disk
27:31 soak it in anything you want as way to test how effective it is
27:36 the microbes. And so um so you would do here is you would
27:42 step one is make a long bacteria your plate. Right? So you
27:47 take a sample of liquid. Just it all over the place. All
27:53 together, right? But before you and let it grow you lay down
27:58 little discs on top right, they'll in pregnant with whatever you want,
28:04 , your favorite disinfectants, whatever. ? Then you lay them down on
28:09 and then you incubate. Okay so can see obviously the areas that are
28:14 are um not clear right all through . This is bacteria that are
28:21 right? But of course you don't any bacteria or not visible at least
28:27 here. Right, clear areas around disk. So chemicals diffuse whatever chemical
28:34 diffuses out of the disc into the um surrounding uh area around it.
28:44 ? And so depending on the sensitivity the microbe it may or may not
28:50 in that area. Right? And how close it grows right to that
28:57 . Whether it's close, right close time. Close. All right,
29:10 more time. My pen is not . Sorry, try this,
29:20 Alright, so whether it's close or away thinking this guy right here that
29:29 no that chemicals has no effect on bacteria grows right to the distance likely
29:36 the thing. Okay um Here's a bit is not much effect either.
29:40 is a big effect. So it's it's a quick and easy qualitative way
29:48 say oh yeah this is may be . That's maybe not. So well
29:51 one forget about it. Right So would obviously do more qualitative assessment after
29:58 on ones that are of interest but just the first pass. How's it
30:03 ? So so not at all what you then you can go into more
30:06 study but very easy way to check . And so uh so the with
30:13 that there's a million ways to test whether it's this method you can use
30:19 and test that in different ways. bottom line is obviously in the absence
30:25 the chemical the cells normally. Right you add chemical do you see a
30:30 ? And that's really the bottom Okay and how much you want to
30:33 into that part of it? You qualitative quantitative. That's that's kind of
30:40 to you. But this is a and easy way to start. So
30:44 a question that relates to that. so again so we have a growing
30:51 that gram positive bacteria we added So here would be so obviously we
30:58 grow this thing we would have prior that if we grow this that we
31:05 where mid log would be. Right the arrows indicating mid log and we
31:11 we add our and that's alright so got it. You would know that
31:22 have done this before and saw Okay grow something like that. So
31:26 would know before where mid lock would . Right? And so that's how
31:30 would add our at our chemical. let me get this eraser. And
31:37 so then um we banned the wait hours, right? So we add
31:46 and then it's four hour interval. we don't know what's gonna happen,
31:52 don't know what the pattern will right? We're gonna be exposed for
31:55 hours then will so will transfer it fresh culture, that's what's going on
32:04 here on the top. Right? we transferred to fresh broth without this
32:10 . Right? So we're gonna do right here, that's what's going on
32:16 there. Okay so for and add , let it go for four hours
32:24 transfer it okay to fresh medium without . Okay and so um so we
32:32 this four times we do that. common to do this at different delusions
32:36 the chemical. Okay. There's a of reasons for that. Probably the
32:42 one is you know why a money thing like you can use it as
32:48 lower concentration, you have to use much etcetera. Okay so here's what
32:52 get right? So in our right which is this one? See
32:58 ? So after four hours of exposure be disinfected measure in terms of growth
33:06 growth right then we look here at subculture. Okay which again we plopped
33:17 from transferred it from here and here see what happens. So this knowledge
33:26 , what is likely? How would classify this um disinfected? All
33:34 but let me open it again. , it's right again. Alright.
33:40 . All right, keep going, going. So how would you classify
33:45 ? Yeah, until again exposing four . Take it out fresh medium without
33:52 affecting what happens? Right, Oh okay, you get that.
34:21 . All right, counting down from . Okay. Let's see here.
34:50 . Alright. So uh it's obviously static because because um as we so
35:05 what we're doing here at this point this sample is asking we've exposed ourselves
35:14 disinfected. Okay. And we saw from most of the delusions we have
35:23 no sorry. We have growth no . Okay, so um right
35:31 Alright. No, gross. So we're asking okay what happened? What's
35:37 state of those sets? Are they they still alive? Are they are
35:44 dead? Okay. And that's what transfer to fresh broth was about,
35:49 ? So we put them in fresh without any disaffected to give them a
35:53 if they are where they grow. so we saw that of course that's
35:58 happened. Right? So that leads to believe it's got to be a
36:03 static agent because they weren't killed. were just kind of growth inhibited.
36:11 yeah this is just a quantitative Ok. Gives us a quick and
36:17 . Okay. Plus minus it did us to figure out that this solution
36:22 really no good. Okay that was dilute to get an effect. Uh
36:27 so we can explore this further of getting quantitative and getting viable counts and
36:34 not to see what's actually going But from this from what you see
36:36 you can make the assumption that your . Okay? Um Now similarly we'll
36:45 back look back at this one. if we were to um look here
36:54 could we say in this clear area this a bacteria static or bacterial seidel
37:01 ? Could you determine that? Just at the plate? No you can't
37:07 the plate. Oh yeah that's a static asian respectable violated. Yeah it's
37:11 a qualitative results. So you have do some further study. You do
37:15 it affected the effect of the micro in order to get that information you
37:20 to do some different type of Okay But again when you're doing this
37:24 of stuff, particularly screening a bunch these at one time. So the
37:28 pass is always kind of a qualitative to do it because it gives you
37:35 quick answer to at least at least tell you what to explore further and
37:38 not to keep testing. Okay um questions about that. So um let's
37:50 at so we'll get into some more on types of agents. Um So
37:57 you might guess you know you expose added this incitement or antiseptic or a
38:05 of some kind to microbe. What's going to affect? Potentially affect the
38:09 you would think? Right, proteins and nucleic acids themselves and that's
38:14 they do. Some are more specific certain targets than others but they'll have
38:20 effect on all of these. Whether it's the membrane proteins of course
38:28 are damaged when you mess with their structure. Right? Or co ordinary
38:35 . So being a protein but you it to unfold the nature.
38:39 Same with nucleic acids. Right. even go as far as breaking
38:45 Okay. That can be done with radiation. So um so it's a
38:50 of things these chemicals and treatments Okay so um so we'll look first
38:58 physical agents and looking at temperature in ways. So both hot and cold
39:07 not everything can be uh huh. every kind of component can undergo temperature
39:16 things are affected by that. So have to use other methods. So
39:20 like filtration radiation. What happened? so here we're focussed on temperature high
39:27 . Right so the autoclave this is like standard conditions 15 P.
39:33 I. 421 to B. Or 15 or 20 minutes you see
39:38 . But it's the uh just the The operative part is the 15 and
39:45 21. And so right here. so steam under pressure gets you the
39:54 that microbes don't ordinarily are never exposed even a hyper thermal file. Okay
40:01 when you're sterilizing something hypothermic file is gonna be of any concern because it's
40:06 gonna be in whatever you're trying to , I'm pretty sure. Okay But
40:11 so the uh it creates also a heat and that's what penetrates in those
40:18 . And so that's why autoclaves are effective in killing and those spores.
40:22 so of course you can boil. so there are equivalent treatments right?
40:28 autoclave sterilized so boiling for 10 Uh hot air. So oven basically
40:34 what that is convection oven of course a longer period of time. But
40:39 can sterilize with this. Um Then gonna be other more milder, relatively
40:47 free. So pasteurization. These were for foods and beverages uh as a
40:54 gentler way of reducing my criminal numbers at the same time keeping the flavor
41:03 texture etcetera of of the product because the manufacturer wants to maintain that right
41:11 know we're out of milk. Trust that look and taste horrible. Okay
41:16 you have to find other ways to that part of the food And and
41:20 yet get the reduction of microbes. so that's what pasteurization is also.
41:26 and so uh so you need to short uh temp long time. I'm
41:31 high temp short time or low temp time. Okay. And these two
41:37 been around for quite some time. . It's the ultra high I think
41:44 much it's there all these are almost with each other. There's some really
41:50 differences. But nonetheless it's a very time. Right in high tech.
41:54 this is a more relatively recent Okay. And it's proven to be
42:01 for areas of the world because not has a fridge. Okay. So
42:06 are particularly useful in allowing a product be that undergoes alter pasteurization to have
42:14 long shelf life, right? Without . Well, once you open then
42:19 ticking, but it can last on on a show for six months.
42:24 this is for you don't get regular . It's been quite useful.
42:30 And you know with all these methods well, there are indicator organisms.
42:38 specific for what they are looking Okay. So for example, with
42:43 , if you wanted to make sure is working fine. Okay. It's
42:48 reports that the so you just get a bacillus bacillus cultures are used for
42:54 standardization to see if it's working right milk pasteurization. It's very common to
43:00 this one. This has a cock . L. A. Has a
43:04 think among the highest known resistances to but they don't form. And those
43:10 . Right so they have a parameter measuring the pasteurization method on these organisms
43:15 make sure they can reduce their numbers . Um Now the cold temp
43:24 cold temp does not kill typically slow down. Okay. And um you
43:32 refrigerated foods right? To prevent spoils ? Provided you know as long as
43:39 can because it uh it slows the down my coach. And some aren't
43:46 are inhibited by um the preservation, ? So we in the lab we
43:54 minus 80. I've used minus 20 minus 80. You can preserve
44:00 You have to kind of put him like a uh an antifreeze, so
44:03 speak. Typically in glycerol to prevent one thing's freezes the ice crystals that
44:09 to actually kill. So if you gently freeze and that's what use like
44:15 or something similar to kind of prevent . And we've had bacteria in minus
44:21 for like 2017 6 years that I still revive. So quite um effective
44:29 that. But you know in terms food uh refrigerating food, there are
44:38 is a type that actually grows refrigeration listeria, we'll talk about that at
44:44 end of the semester in the context diseases. But um it's found on
44:52 of process like Delhi needs your your and ham alone and salami. Um
44:59 the like and uh it's we've likely have all had hysteria. I'm notorious
45:07 eating foods path through exploration date so to the annoyance of my wife.
45:12 uh I mean, I'll never really sick from I don't go to extremes
45:18 it's very slimy or something. And . Um but it's why for most
45:24 us have healthy immune systems on an . But pregnant pregnant women do have
45:29 be America. Right? And so it can affect the fetus, listeria
45:34 so um so it's practice for pregnant to not eat these kinds of foods
45:42 pregnancy. Okay, um now So again, not everything can hold
45:48 temperature. So we use filtration. call label liquids which are sensitive to
45:55 high heat. Uh so uh very . Really used to use 0.2 micron
46:02 . All the 0.45 will will remove bacterial types. Um 0.2 are generally
46:11 . Um but they don't really can't get rid of viruses. Oh,
46:17 those aren't really a concern. Typically your filter sterilizing. Uh the
46:27 And we have media in a lab can't be autoclaves. So we have
46:30 use filter sterilization for it. So certain things that use it for um
46:36 , radiation radiation um as I'm you know, as you look at
46:44 electromagnetic spectrum, we're interested in wavelengths are kind of on this on this
46:54 . Okay. To the right, , over here and beyond.
47:03 Less than that. So that's UV branch. 200 to 80. And
47:08 even lower. Right? So remember equates to wavelength shorter wavelength more
47:13 Okay. And so you be Non ionizing radiation and gamma rays.
47:20 rays ionizing radiation. Okay. So you'd be like uh can be effective
47:28 uh surface disinfection. We call We have a biosafety cabinet. We
47:36 culture work in as a as a light. And we turn it on
47:39 night to zap the surface, To kill anything that's on there.
47:43 it kills through mutating the cells based in D. N. A.
47:50 create enough of these. Of course can be lethal. Um But you
47:55 , many things stop UV light a plastic Petri dish that can stop
48:00 light. So uh to get more of penetration if you will uh gamma
48:06 X rays time. So you can the difference in wavelength to 300 nanometers
48:13 less than 3000.1. So, super energy and can generate these kind of
48:18 radicals you see here. Okay. fragmenting pay gas. So it's quite
48:25 . And it has it's gotten more more traction I guess as and and
48:34 um use on food frozen foods like chickens and things. Uh radiation is
48:40 common nowadays to obviously the danger there food borne pathogens using radiation to zap
48:47 uh very briefly obviously cause you don't to cook the frozen chicken cook the
48:52 . But they do use that industry that purpose. Um as well as
48:56 like uh plastics and other types of you wouldn't use radiation for liquids.
49:08 radiation could probably to a degree, it's uh it's also why you wear
49:13 lead apron. Right? Because it's powerful radiation. Um Okay, so
49:21 agents probably familiar with a lot of . So again, I'm not getting
49:26 in the weeds and super detail on kind of like, here's here's some
49:31 , there's kind of in general terms they do. Nothing more than
49:35 Okay, so they're phenolic six are compounds. So you see like over
49:42 , okay, these tend to be volatile. More, you know,
49:46 you apply them, can they hang for a bit? Okay. But
49:50 all they all three have in common proteins. DNA is lifted. So
49:55 of a range of targets here. , beta nine. Is that yellow
50:00 ? You probably seen your doctor's office wash hands with um I also is
50:06 The alcohol. So ethanol, we ethanol in the lab disinfect bench tops
50:14 it turns out that water does make difference. Right, so it's actually
50:18 ethanol Is more effective than 95%. , so, so alcohol is kind
50:26 help dissolve membranes, they get inside water helps to be more effective at
50:31 . Okay, so you got a bit more water to it. That
50:34 increases its its efficacy. Okay. so detergents. So this is a
50:43 these are called. Co ordinary means think they're called. But they have
50:48 common structure of being very long hydrophobic if you will. So that really
50:55 a fossil lipid that allows them to membranes which I um gasses.
51:02 So gasses aren't good for liquids. penetrate very brilliant liquids. But for
51:09 like plastics, your pipette tip boxes boxes, pipette tips, Petri
51:15 These things are often uh gasses are for that. Monoxide is the one
51:20 choice uh and it can be a agent for sure. Um as well
51:27 things like syringes, tubing etcetera. so what happens is it um in
51:33 presence of acid or base is what the kind to be really reactive forming
51:40 kinds of charged species. Okay. then those interact with proteins and gasses
51:47 cause damage. And so they can quite effective in in kind of what
51:51 used for which basically plastics of different and and these kinds of solid structures
51:59 you will. Right so um okay they're resistant. So because disinfectants attack
52:12 targets in itself, it's not common um bacteria to become resistant to.
52:21 they would have to accumulate enough mutations be able to counteract every target that
52:27 disinfectants or treatments are generating in the , it's not common. The only
52:33 it can be a problem is if then use that say for example
52:39 a very low concentration as you lower concentration of disinfectant below what you should
52:47 using. Okay. The manufacturer recommends the number of targets is less for
52:54 disinfecting. And then potentially mutations can that allowed to be resistant to
53:00 This chemical back here. This Right. This one is found in
53:08 found in a lot of hand Ok. It's and it's just been
53:14 because it was being put in very concentrations of bacteria became resistant to
53:20 So it can happen again if you you really minimize the concentrations of these
53:26 . Now, in contrast, antibiotics we have single parts. Right?
53:35 it's a um an enzyme that's part a process like several synthesis or Viber
53:43 subunit. Right? Protein synthesis. they typically all have single parts.
53:50 ? So it's not uncommon that, know, take a single mutation occurs
53:56 makes it resistant. Okay, of course that doesn't happen. What
54:02 is the situation is the constant exposure antibiotics because they're everywhere right there in
54:09 food we eat there in um they're the water. Right. Take
54:15 I think data where samples are taken different water samples um from sewage and
54:22 amount of antibiotics are like nuts. , so of course it's the presence
54:28 those that sets the stage for resistant . Right, Okay. Natural
54:36 Right. So we can minimize Okay. And minimize indiscriminate use about
54:45 other than that that can go a ways. But uh but of course
54:51 easier said than done I'm thinking but the we'll talk more about antibiotics veteran
54:59 but I'm only gonna I'm only showing just for illustrative purposes. Right?
55:04 the mechanisms of resistance. So it's . What you might think right if
55:08 have a bacterium and here's antibiotic, can it do to become resistant?
55:15 it can completely obliterate. Let's just at the diagram right? You can
55:23 this basically just destroy and activate the did too or whatever. Right?
55:31 just inactivated. Okay. Um It just say let's not let it come
55:37 to the cell. Okay. So things typically come in through various types
55:42 Torrance you know on the surface there's mutation occurs that. Now the specificity
55:48 commit to the cell. Alright, way is alter the target.
55:56 That was the right resistant. So to that. Halloween on the on
56:05 peptide cross bridge. Well it mutates now it's not alan there is something
56:09 you've altered the target. So now becomes resistant. Right? And then
56:14 then you can also pump it Alright that's another mechanism. So the
56:20 we talked about you know the cells cells kind of just stopped growing.
56:25 ? So so having um growth is not always for every antibiotic I'm finding
56:33 active growth, the antibiotic works But And so the bacteria is simply
56:38 not grow, right? And then antibiotic concentrations dissipate and it begins to
56:44 . So all different types of Okay. But it's why right?
56:50 we have to constantly having to find modify, modify what we have to
56:56 kind of tweak it somewhat. So definitely a war. And uh lastly
57:04 other other kind of ways besides chemicals. Right? What can we
57:11 ? Well, we could boost what already have. Alright, so probiotics
57:19 your own microbiome is really acquire your system. It does help your immune
57:25 . Okay. Uh So boosted with . If you are on antibiotics for
57:33 reason or system suppressed somewhat, then probiotics can help that. Okay.
57:44 And finally face Therapy. I think is becoming thing right? Is this
57:51 here? Um It's so we'll start about this on thursday. But fade
57:59 bacterial viruses. They're specific for bacteria there are species specific. Okay.
58:07 so there was a case and I it here or not. Um
58:13 An article here called Face Therapy. had no idea this has been going
58:17 for like 100 years. Okay. 100 years ago they didn't know as
58:21 about faith. The guy that discovered . This guy uh This is looking
58:26 19 hundreds, 1910, 20 Of course Germ theory was well known
58:32 then we knew forward diseases he discovers that they infect bacteria. Put two
58:38 two together. Right, you fade kill these infectious bacteria makes sense.
58:44 they weren't really up to at this . You really had a very well
58:50 fage for mass production and I don't know all, there was no
58:54 So it kinda had mixed results but idea the idea kind of waned.
59:00 or they were actively working on it then it comes back really more
59:05 Okay, so this person here, were both on vacation in Egypt and
59:13 guy comes down with this disease. caused by a senator Baxter.
59:20 And there's no antibiotics to control So she scans the internet and saw
59:26 on page there. So they actually to the lengths of finding a page
59:32 would in fact this bacteria. And took like there were people that of
59:38 study page and they have like libraries cultures of page maybe end up having
59:44 to isolate from with the sisters different hunt which included coming through uh I
59:53 new faces from sewage barnyard waste, of navy ships. They finally found
59:59 and after taking the page improved almost . Right? So this has like
60:08 I think 13. So this is really spurred on again and it's logically
60:13 makes a lot of sense. Very specific in terms of the the
60:18 agent. Finding the agent. I believe that for every living thing out
60:22 there's a there's a virus that affects , Right? And so of course
60:27 lots of bacteria fades and so I this is the coming thing. Uh
60:32 think it's the right direction to But there's there's lots of lots of
60:36 here that have to be worked out because bacteria can become resistant. So
60:41 have to have that to to So but certainly I think a promising
60:47 to go in terms of fighting these infectious agent, especially with the level
60:52 antibiotic resistance we're seeing nowadays. So anyway I just want to throw
60:56 in uh the uh I think good . So alcohol early and uh again
61:13 have any questions you can email Come office hours. Uh
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