Hello everyone, I calculated the standard rate constant of Tb³⁺ at the liquid Zn electrode in LICl-KCl melt by CV. The result is about ~10^-4 cms^-1. I found some standard rate constants on the inert electrode in various molten salt, which these values are calculated to be 10^-2 ~ 10^-3 cms^-1. And it makes me wonder that this parameter at liquid Zn electrode is smaller than that on the inert electrode. Is this normal? What is the real reason for the  case? Thanks!

Dear all,

I finished my analyses and those are my results (picture). As you can see, I have basicly two groups, blue and yellow. Blue group contains less number of samples and it looks like it's more influenced by factors  6/13. Second group contains at least 23 samples and it's more influenced by combination of factors 2/6/7/18. Could this be because of number of samples?

(All species are from one genus.)

I really don't know what to think, so if someone could help, I will be glad.

Dear all,

I am searching the soft copy of the book 'Grey Data Analysis
Methods, Models and Applications' http://www.springer.com/la/book/9789811018404 for one of my students for educational and research purpose only.

It would be appreciated if you provide me this book. I can be reached at syed.mithun@gmail.com.

Regards,

Dr. Syed Mithun Ali.

Is there a consensus on the optimal concentration of glutaraldehyde for the preservation of marine phytoplankton?  I typically use 1%, but notice that other researchers use from 0.1% to 3%.

I am interested in maintaining as many taxonomic features as possible for LM and SEM with the lowest concentration of glutaraldehyde that is acceptable, since I don't like working with this chemical at sea. I typically work in low chlorophyll high nutrient areas of the Southern Ocean, but may find sea-ice blooms from time to time.

I appreciate you thoughts and recommendations :).

Hi.

I'm working on a new project which involve "quantify" an effect on protein levels. As I am working with rat samples I have a lot of samples to pass through Western blot.

In my previous lab I never had the chance to perform this step so right now I have a lot of questions. I wonder if I can compare different blots and how ?

And I have to say that for some of my proteins I use different exposition time for the same membrane (I cut the membrane in different pieces) and depending on saturation. I try to be at the maximum signal before any saturation but for some of my protein of interest I can say that it will never be the case (signal too faint). Am I doing right ?

Should I present my result as ratio of protein of interest on loading control and only then compare them. Or should I compare membrane per membrane and then mix all the results ?

I don't know if I am being clear...

Thank you

I know there is a lot of discussion on the definition of rare species and I also know of some ways or rules of thumb to define them, but I was wondering what researches commonly use. My question arises from a dataset containing species (larval dragonflies) densities of 201 sites. I know of lower quartile rule of ordered occurrences or just defining rare species by stating that all species are rare that occur in less than e.g. 5 sites of 201 or something similar. But what methods do you use?

Regards, 
Daniel

I want a program for drawing maps and charts

I am trying to purified a PCR product from gel extraction (2% agarose), for the purification I used PureLink Quick gel extraction and PCR purification combo kit (Invitrogen). And for the PCR reaction I used Go Taq Green Master mix from Promega.

The purification purpose is for sequence. After the purification I made a electrophoresis. The electrophoresis conditions: 100V, 30min, 2% agarose. I used blue/orange loading dye and GelRed for staining. 

As a result I got the expected bands but I also have anomalous bands in the superior part of the gel, can these be form from de loading dye? or green master mix? will this affect the results form sequencing? 

Hello all, 

I'm very new to research, and science in general. I just started in my first lab two months ago, so I don't have a lot of experience. 

I'm currently analyzing western blot data. My PI and I are having some disagreement as to the best method to normalize the protein of interest (Neuropsin) to a total protein stain using Ponceau S.

When doing densitometric analysis with AlphaView software of the Ponceau stain, I quantify the total protein for each sample using the entire lane (meaning I make the box to be analyzed around the whole lane). My PI tells me that I should be using only a small band from each lane instead of the whole lane. But it seems to me that this defeats the purpose of quantifying the total protein for each sample because it only quantifies a portion of the total protein. If I'm analyzing the entire band of my protein of interest, but only a portion of the total protein, it seems that the data from normalization won't be reliable. 

Not much literature actually reports densitometric techniques, but in the papers that do, it appears that most researchers are using the entire lane to quantify total protein. Could anyone help clear this up for me? I want to make sure I'm using the most reliable methodologies.

Thank you all ahead of time, I appreciate any responses. 

I am using visual seminars to address functional illiteracy at both an undergraduate down to a middle school level. I have found that images have the ability to undercut illiteracy. Visual metaphors seem to be one of the most effective tools for doing this.

I want to learn the COMSOL (5.2 a) Acoustic Module. If anyone has the tutorial guide or know some web links to learn that.

Please share with me, I shall be very thankful to you.

I am designing a glass beam with glass panels attached to each other with a DeloPhoto Bond adhesives. Further I am prestressing the 12.7 mm strands.

I am modeling this with 1 strand and 2 strands and my 1 strand beam is resisting more force than the 2 strands beam.

I am using Abaqus as a FEA package.

What can be the reason to that?

Currently I am working on NO₂ satellite data in molecules/cm² . But I don't know how to convert it to ppm (parts per million). I would be grateful if anyone can give me some suggestions. Thanks

Servant leadership is often presented as having positive impact on employee behaviour and corporate performance.
I wonder if this positive impact is absolute or depending on dominant culture and values.

The equipment we have is Agilent HPLC(with UV detector only). There is a paper in 1985 that uses UV-HPLC (195 nm) to detect 2-DG but uses NH2 column which we don't have. Is there any alternative to solve this issue and find the  concentration of 2-DG by some other technique?

There are ample papers that uses HPLC combined with other detection techniques that doesn't match our equipment, so i am in search for some simple, convenient, and reliable method which can determine concentration of 2-DG. Thanks in advance.

I am looking at the influence of higher level managerial capability ( Leadership) in relation to dynamic capabilities. need some suggestion and recommended papers for reference in developing a measurement scale for this capability .   

Can we say that Motivational Interviewing, problem-solving, and self-monitoring are the techniques of CBT? or they are separate techniques? I am bit confused, I have read articles collectively called CBT of these three techniques. While some articles used Motivational Interviewing as a separate technique. Please guide.

I heard that three researchers are needed to finalize the selection of articles that will be included in a meta-analysis, is this typically true in the field?

Can we prepare plants extracts in ethanol and chitosan in distilled water ? or this is necessary to prepare both in distilled water ?

I would like to simulate the injection and in cylinder flow of the engine and further expand to simulation of combustion. 

Are there free/open source softwares that could be used for this purpose? 

The goal would be to acculturate sojourners via indigenous sociocultural constructs. 

Hello,

I am interested in observing stained (with ORO solution) isolated lipid droplets with light microscopy and I have seen that collagen could be of a use. However, the paper I found does not mention clearly which company provides it or what type they have used. Does anyone have any idea? 

Thank you in advance

hey guys , Would you like to share your RNA extraction protocol?

I've been in different lab and find there are lot different between the protocol.

Usually the all step performed on the ice

first step is add trizol, mixed well and stand for few mins,

add chroloform, votex and stand for few mins, 

centrifuge and trasfer supernant on new tube

add isoalchol and revert, store at -80℃ >30mins or just stand on ice

centrifuge and remove supernant

wash with 80%alcohol for two times

dissolve in RNAase free water.

what's ur centrifuge speed and time? do you guys store at -80℃?

Hi. This is to anyone who has ever observed the same. We found a large Indel (400bp) within a known gene. When the insertion is not present (deletion), the gene is expressed (like a functional version of the gene). But when the insertion is present, there is a SNP within the inserted sequence that can also be correlated with the expression. Something like this:

Deletion --> expresion

Insertion:  SNP A within insertion --> expression

Insertion:  SNP T within insertion --> No expression

The correlation between deletion/expression could be explained as a functional version, and the insertion could disrupt the gene, so it should be non functional (like many transposons do). But having expression even with the insertion, but only when a specific SNP is present, is confusing to me.

I would appreciate any suggestion to find a biological explanation for this results. 

Thank you!

I am doing DSC of PA11 based blend samples wherein I am need to find % crystallinity.