- 2018- James P Allison and Tasuku Honjo for Immune
checkpoint therapy to treatments for advanced, deadly cancers.
- 2017- Jeffrey Hall,
Michael Rosbash and Michael Young for unravelling how bodies keep a
circadian rhythm or body clock
- 2016 - Yoshinori
Ohsumi for discovering how cells remain healthy by
recycling waste.
- 2015 - William C
Campbell, Satoshi Ōmura and Youyou Tu for anti-parasite drug
discoveries.
- 2014 - John O'Keefe,
May-Britt Moser and Edvard Moser for discovering the brain's
navigating system.
- 2013 - James Rothman,
Randy Schekman, and Thomas Sudhof for their discovery of how cells precisely transport
material.
- 2012 - Two pioneers
of stem cell research - John Gurdon and Shinya Yamanaka - were awarded the
Nobel after changing
adult cells into stem cells.
- 2011 - Bruce Beutler,
Jules Hoffmann and Ralph Steinman shared the prize after revolutionising
the understanding of how the body fights
infection.
- 2010 - Robert Edwards
for devising the
fertility treatment IVF which led to the first "test tube
baby" in July 1978.
- 2009 - Elizabeth
Blackburn, Carol Greider and Jack Szostak for finding the telomeres at the ends
of chromosomes.
Wednesday, October 3, 2018
Nobel Prizes for Medicine or Physiology during 2009-2018
Sunday, March 25, 2018
It's Urgent to Protect the Biodiversity in the World
An intergovernmental ecological body said on Friday that the biodiversity, the essential variety of life forms on Earth, continued to decline in every region of the world, significantly reducing nature’s capacity to contribute to people’s well-being.
Those alarming trends are endangering economies, livelihoods, food security and the quality of life of people everywhere, according to four peer-reviewed regional reports released by the Intergovernmental Science-Policy Platform on Biodiversity and Ecosystem Services (IPBES).
Human-induced climate change, which affects temperature, precipitation and the nature of extreme events, is increasingly driving biodiversity loss and the reduction of nature’s contributions to people, said Jake Rice, a co-chair of the Americas assessment.
In the Americas, the populations of species are about 31 percent smaller than those was at the time of European colonization, according the report. With the growing effects of climate change added to the other drivers, this loss is projected to reach 40 percent by 2050, it says.
In Africa, by 2100, climate change could also result in the loss of more than half of African bird and mammal species, a 20 to 30 percent decline in the productivity of Africa’s lakes and significant loss of African plant species.
The most recent sad example went to the death of the world’s only remaining male northern white rhino in Kenya on Monday. Its death left only two female northern white rhinos on the planet.
There have been some good news in Asia, however. Over the past 25 years, marine protected areas in the region increased by almost 14 percent and terrestrial protected area by 0.3 percent. Its forest coverage increased by 2.5 percent, with the highest increases in North East Asia (22.9 percent) and by South Asia (5.8 percent).
But the report considered those efforts in Asia insufficient to halt the loss of biodiversity. Unsustainable aquaculture practices, overfishing and destructive harvesting, threaten coastal and marine ecosystems, with projections that, if current fishing practices continue, there will be no exploitable fish stocks in the region by 2048.
Also in Asia, intertidal zones are also rapidly deteriorating due to human activities as up to 90 percent of corals will suffer severe degradation by 2050, even under conservative climate change scenarios.
In the European Union, only 7 percent of marine species and 9 percent of marine habitat types have shown a “favorable conservation status.” Moreover 27 percent of species assessments and 66 percent of habitat types assessments show an “unfavorable conservation status.”
“One of the most important findings across the four IPBES regional assessments is that failure to prioritize policies and actions to stop and reverse biodiversity loss, and the continued degradation of nature’s contributions to people,” said Anne Larigauderie, the Executive Secretary of IPBES.
“Tools like these four regional assessments provide scientific evidence for better decision making and a path we can take forward to achieve the Sustainable Development Goals and harness nature’s power for our collective sustainable future,” said Achim Steiner, Administrator of United Nations Development Program.
Wednesday, February 14, 2018
Stem cells that produce sperm use a genetic trick to stay perpetually young across generations, researchers at the University of Michigan (UM) Life Sciences Institute have discovered.
The results have been newly reported in the journal eLife.
Certain sections of the fruit fly genome get shorter with age. But remarkably, some reproductive cells can repair the shrinkage, and this genomic shrinkage may underlie aspects of aging and hint at ways that select cells might thwart it.
In the study, UM researchers focused on workhorse genes encoded in ribosomal DNA, or rDNA. These genes carry instructions for the parts that make up ribosomes, cellular machines that turn RNA molecules into every protein needed in the body.
In fruit flies, chains of rDNA genes are found on the X and Y chromosomes. Compared with young male fruit flies, old males had a shortage of rDNA genes on the Y chromosome, leaving them with a shrunken Y chromosome.
Moreover, this dearth of rDNA seems to be passed on from generation to generation. Geriatric fly fathers, those 40 days old, passed on their reduced number of rDNA genes to their sons, UM researchers found. These sons had considerably fewer copies of rDNA genes than sons born to younger fathers.
Then the researchers saw something surprising. In many cases, this rDNA loss reversed itself. At about 10 days of age, sons born to old fathers had recovered enough rDNA to be comparable to sons born to young fathers.
"This recovery was something we really didn't expect," said UM Life Sciences Institute faculty member Yukiko Yamashita.
The results suggest that rDNA rejuvenation in sons might be a crucial aspect of how stem cells persist from father to son. The researchers do not yet know whether such a reset can happen to female stem cells in the ovaries.
Until now, researchers had observed the phenomenon only in yeast. If the results hold true for humans, they could offer insight into how most cells deteriorate over time.
Being pushed, Yamashita would wager that some types of immortal cells in people can perform the same rejuvenating trick to prevent the rDNA declines that come with age.
My God, Inout Scripts Adserver is full of errors and warnings
I checked the Inout Scripts Adserver
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Nair and Saranya.
In addition, most of the addons are
not working at all.
The inoutscripts software has
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These Inout Scripts Scammers had
never got these bug fixed. They just took cash and left me nothing working.
Monday, February 12, 2018
Recombinant DNA technology
Recombinant DNA technology, joining
together of DNA molecules
from two different species that are inserted into a host organism to produce
new genetic combinations that are of value to science, medicine, agriculture,
and industry. Since the focus of all genetics is the gene, the fundamental goal
of laboratory geneticists is to isolate, characterize, and manipulate genes.
Although it is relatively easy to isolate a sample of DNA from a collection of cells, finding a
specific gene within this DNA sample can be compared to finding a needle in a
haystack. Consider the fact that each human cell contains approximately 2
metres (6 feet) of DNA. Therefore, a small tissue sample will contain many
kilometres of DNA. However, recombinant DNA technology has made it possible to
isolate one gene or any other segment of DNA, enabling researchers to determine
its nucleotide sequence,
study its transcripts, mutate it in highly specific ways, and reinsert the
modified sequence into a living organism.
DNA Cloning
In biology a clone is a
group of individual cells or organisms descended from one progenitor. This
means that the members of a clone are genetically identical, because cell
replication produces identical daughter cells each time. The use of the word clone has
been extended to recombinant DNA technology, which has provided scientists with
the ability to produce many copies of a single fragment of DNA, such as a gene,
creating identical copies that constitute a DNA clone. In practice the
procedure is carried out by inserting a DNA fragment into a small DNA molecule
and then allowing this molecule to replicate inside a simple living cell such
as a bacterium. The small replicating molecule is called a DNA vector
(carrier). The most commonly used vectors are plasmids (circular DNA
molecules that originated from bacteria), viruses, and yeast cells.
Plasmids are not a part of the main cellular genome, but they can carry genes
that provide the host cell with useful properties, such as drug resistance,
mating ability, and toxin production. They are small enough to be conveniently
manipulated experimentally, and, furthermore, they will carry extra DNA that is
spliced into them.
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Inout Scripts Review: Advantages and Disadvantages
https://www.sitejabber.com ›
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Forums › The Digital Point › General Chat
Friday, February 9, 2018
E. coli Transformation
Long
1) Get 200ul aliquots of E. coli
(DH5a for normal transformation or DE3 for expression) from -80C freezer and
let thaw on ice.
2) Add DNA
For plasmid: 1ul DNA desired
For ligation: 10ul ligation reaction
-Also include a negative control
with no DNA.
3) Incubate for 30min on ice.
4) Heat shock for 90sec at 42C.
5) Incubate for 1min on ice.
6) Add 1ml LB.
7) Agitate at 37C for 45min – 2hrs
(1hr is good).
8) Spin down and pour off LB leaving
~100ul.
9) Resuspend cells in the ~100ul.
10) Plate the entire suspension on
appropriate prewarmed plates.
11) Incubate at 37C overnight.
Short
Note: Use for amplifying AmpR
plasmids only.
1) Get 200ul aliquots of E. coli
(DH5a) from -80C freezer and let thaw on ice.
2) Aliquot 50ul of cells into tubes.
3) Add 1ul DNA desired.
4) Incubate on ice 5min-30min.
5) Plate on prewarmed LB-Amp plates.
(Plate the whole thing--no spinning, no nothing).
6) Incubate at 37C overnight.
Blue/White Selection
-Used for plasmids like Bluescript.
-No insert=Blue. Insert=White.
-Do long transformation of ligations
basically as described above.
-While cells are agitating,
A) Spread X-Gal and IPTG on plates.
X-Gal (50mg/ml): 20ul
IPTG (1M): 10ul
B) Incubate at 37C to dry (about
30min).
E. coli Miniprep
1) Grow 2ml culture o/n.
2) Spin down. Pour off all but
~100ul of sup. Resuspend cells in the ~100ul.
3) Add 130ul P1. Resuspend.
4) Add 130ul P2. Mix immediately.
5) Add 182ul N3. Mix immediately.
6) Spin 10 min at 4C. (Removes
genomic DNA and debris).
7) Transfer sup to a fresh
eppendorf.
8) Add 900ul ice-cold 100% EtOH
(bottom shelf in door of -20C freezer). Mix thoroughly.
9) Spin 15min at 4C. Discard sup.
10) Wash pellet once with ~400ul
ice-cold 70% EtOH.
11) Dry pellet on rack or in
speedy-vac.
12) Resuspend in 50ul water. Use
3-10ul for digest.
Bioprotocols of Molecular Biology
One-Tube Isolation of DNA from Mouse
Tails
Michael R. Green
and Joseph Sambrook
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot093534
Buffers
Michael R. Green
and Joseph Sambrook
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.top098210
Caring for Escherichia coli
Michael R. Green
and Joseph Sambrook
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot101337
Protein Immunodepletion and
Complementation in Xenopus laevis Egg Extracts
Christopher Jenness,
David J. Wynne,
and Hironori Funabiki
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot097113
Analysis of Mitotic Checkpoint
Function in Xenopus Egg Extracts
Yinghui Mao
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot099853
Transformation of Schizosaccharomyces
pombe in a 96-Well Format
Assen Roguev,
Jiewei Xu,
and Nevan J. Krogan
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot091942
DNA Preparation from Schizosaccharomyces
pombe
Assen Roguev,
Jiewei Xu,
and Nevan J. Krogan
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot091959
Preparation of Plasmid DNA by
Alkaline Lysis with Sodium Dodecyl Sulfate: Maxipreps
Michael R. Green
and Joseph Sambrook
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot093351
A Single-Step Method for the
Simultaneous Preparation of DNA, RNA, and Protein from Cells and Tissues
Michael R. Green
and Joseph Sambrook
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot093500
Gateway Recombinational Cloning
John S. Reece-Hoyes
and Albertha J.M. Walhout
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.top094912
Propagating Gateway Vectors
John S. Reece-Hoyes
and Albertha J.M. Walhout
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot094920
Generating an Open Reading
John S. Reece-Hoyes
and Albertha J.M. Walhout
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot094938
Using Multisite LR Cloning to
Generate a Destination Clone
John S. Reece-Hoyes
and Albertha J.M. Walhout
Cold Spring Harb Protoc 2018; doi:10.1101/pdb.prot094946
Preparation of DNA from Embryonic
Stem Cells or Other Cultured Cells
Richard Behringer,
Marina Gertsenstein,
Kristina Vintersten Nagy,
and Andras Nagy
Cold Spring Harb Protoc 2017; doi:10.1101/pdb.prot092718
Analysis of DNA Methylation in
Mammalian Cells
Paul M. Lizardi,
Qin Yan,
and Narendra Wajapeyee
Cold Spring Harb Protoc 2017; doi:10.1101/pdb.top094821
Methylation-Specific Polymerase
Chain Reaction (PCR) for Gene-Specific DNA Methylation Detection
Paul M. Lizardi,
Qin Yan,
and Narendra Wajapeyee
Cold Spring Harb Protoc 2017; doi:10.1101/pdb.prot094847
Methyl-Cytosine-Based
Immunoprecipitation for DNA Methylation Analysis
Paul M. Lizardi,
Qin Yan,
and Narendra Wajapeyee
Cold Spring Harb Protoc 2017; doi:10.1101/pdb.prot094854
High-Throughput Deep Sequencing for
Mapping Mammalian DNA Methylation
Paul M. Lizardi,
Qin Yan,
and Narendra Wajapeyee
Cold Spring Harb Protoc 2017; doi:10.1101/pdb.prot094862
Preparation of Single-Stranded
Bacteriophage M13 DNA by Precipitation with Polyethylene Glycol
Michael R. Green
and Joseph Sambrook
Cold Spring Harb Protoc 2017; doi:10.1101/pdb.prot093419
Growing Bacteriophage M13 in Liquid
Culture
Michael R. Green
and Joseph Sambrook
Cold Spring Harb Protoc 2017; doi:10.1101/pdb.prot093435
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Tuesday, February 6, 2018
Cloned monkeys could help development of drugs for human brain diseases
Chinese scientists' successful cloning of monkeys could eventually help the development of new drugs to treat human diseases, like brain and nervous system problems, a leading Chinese neuroscientist said.
At the end of 2017, a non-human primate research facility under the Beijing-based Chinese Academy of Sciences (CAS) produced two cloned macaques.
Allaying fears that cloning monkeys for research could ultimately lead to human cloning, Poo Muming, director of the Institute of Neuroscience at CAS, told Xinhua, "We have no intention to clone humans."
The macaque cloning was done for a humane reason, he said: "Because this is the species that will really help human health and cure human disease."
The cloning will reduce the use of large numbers of primates for research, especially in the West.
In 2016, the United States used over 71,000 primates for research or experimentation, according to the U.S. Department of Agriculture's animal and plant health inspection service.
U.S. pharmaceutical companies import at least 50,000 monkeys every year to test the efficacy of different drugs and determine safe doses for human clinical trials, Poo said.
"That is a huge number of monkeys used, which you should consider unethical," he said.
Since these monkeys have diverse genetic backgrounds, researchers must use a large number to make sure that the observed effects are due to treatment and not because of the genetic variation.
"Cloning is really the way to go," Poo said. "Because it reduces the interference (of) the diversity of genetic background on drug development. So it is for (that) ethical reason that we (have cloned) monkeys."
Darren Griffin, genetics professor at the University of Kent, holds the same view.
"If they can produce these cloned animals that means that you could use fewer animals for ... research, rather than the number being used at the moment," he said in a previous interview with Xinhua.
At present, the medical community mostly uses mice as a model to research cures for human diseases. But for many diseases, especially brain diseases, drugs that are developed using mice as model have failed clinical trials in humans, Poo said.
"Basically all big pharmas have given up developing neuro drugs," he said, citing two decades of drug development failure, with hundreds of billions of dollars spent on each drug.
"Next, we want to develop clones of animals that carry brain disorders," he said, especially degenerative or development diseases that have clear genetic causes.
Poo said he would like to focus on Alzheimer's, Parkinson's, autism and ALS, a nervous system disorder that causes disability.
Regarding the debate on the ethics of non-human primate cloning, he said every new technology is a two-edged sword: "There will be discussions and we'll see how the society deals with it."
In the 1970s, when genetic engineering technology first came out, he said everybody was worried about its harmful effect on humans.
"But so far, it has been 40 to 50 years and you don't see any real problem yet," he said.
"Cloned monkeys could be very valuable in studying specific aspects of human disease," said Tom Holder, director of Speaking of Research, an international organization that supports the use of animals in scientific labs.
"The breakthrough has shown that it is possible," Holder said in an emailed interview to Xinhua. "But it is too early to make any conclusions on whether the method will be able to be repeated efficiently and reliably."
Holder also said non-human primate research is subject to increased ethical and welfare considerations and is generally used only when other species are unsuitable for the research.
Tailed spider trapped in 100-million-year old amber offers insight in evolution
A spider-like creature bearing a long tail has been discovered in an amber from Myanmar dating back about 100 million years.
"There's been a lot of amber being produced from northern Myanmar and its interest stepped up about ten years ago when it was discovered this amber was mid-Cretaceous," said Paul Selden, a palaeontologist at the University of Kansas and an author of a paper on the ancient arachnid.
"Therefore, all the insects found in it were much older than first thought," Selden told the university in an interview.
The finding is published Monday in a paper in Nature Ecology & Evolution by an international team of researchers from the United States, China, Germany and the United Kingdom.
According to the paper, the creature shares many similarities with modern spiders including fangs, eight legs and silk-producing spinners.
Moreover, it also bears a long flagellum, or a tail, at its rear, which is not commonly seen among modern spiders.
Thought the ancient arachnid has a tiny body, only about 2.5 millimeters long, it had a tail nearly twice of its body length.
"Any sort of flagelliform appendage tends to be like an antenna," Selden said, "It's for sensing the environment. Animals that have a long whippy tail tend to have it for sensory purposes."
The tailed arachnid, named Chimerarachne after the Greek mythological Chimera, documents a key transition stage in spider evolution.
Previously, Selden and his colleagues had found similar insects without spinnerets from the much older Devonian and Permian periods.
"That's why the new one is really interesting, apart from the fact that it's much younger -- it seems to be an intermediate form," Selden said.
"In our analysis, it comes out sort of in between the older one that hadn't developed the spinneret and modern spider that has lost the tail," he added.
Most reviewed 13 Inoutscripts Softwares
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If you are a victim of inoutscripts, please don't
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Reviews:
1.
I have used most of these Inout Scripts. I purchased 13 of them.
2.
They are just liars, since they don't have the technology of big
data. The hypertable/Hadoop is not working at all. It would take 50 years to
fill 10 TB storage according to our calculation. The Inout spider can just
crawl about 2000 pages per day.
3.
Some of the inourscripts can cause the server down, since they
produce a ton of error log every day.
4.
The sites are super slow. They will blame you whichever servers
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5.
The inout search engine is not compatible with inout spider. It
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6.
The inout scripts are not SEO. You can just get little traffic
however you try.
7.
The webportal is not working. You'll never get something like
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8.
The cronjob of inoutscripts adserver is not working. The addons
are not compatible.
9.
The inout articlebase has injection defects.
10. The inout celebrities is
not responsive design. If you need a mobile mode, they will charge $480-800 as
customization.
11. The inout queryspace is
still using PHP 5.4 which is not supported by the official site.
12. The webmail ultimate can't
be used to send or receive emails. It is a knid of malware that will get
security warning from chrome and google.
13. I purchased 4 APPs, but
they did not give me any one.
14. You can log into the inout
socialtitles but can't log out from it sometimes. It does not have an email
confirmation and recap feature. If you need these functions, they will charge
you for customization. My site were attacked and spammed repeatedly.
15. They never refund you once
you transfer the $$$. Yes, you'll never get any effective support from the
staff.
16. Just a few of them here.
I'll tell you uch more bugs and errors of Inout Scripts later.
The below are all the InoutScripts:
21 scripts in over 115 countries
All Advertising Solutions Search Solutions Email
Solutions Portal Solutions Mobile Apps
Inout
Search Engine
Meta Search Engine Script with multiple API support. Google Clone.
Inout
Search Engine
Meta Search Engine Script with multiple API support. Google Clone.
Inout
Spider
Powerful Web Crawler Script. A Googlebot Clone for Small/Medium Business
Spider
Powerful Web Crawler Script. A Googlebot Clone for Small/Medium Business
Inout
Site Search
Fast & Simple Site Search. Let visitors find what they are looking for. Quickly!
Site Search
Fast & Simple Site Search. Let visitors find what they are looking for. Quickly!
Inout
Adserver
Ad serving & Ad Management Script. Adwords & Adsense Clone.
Adserver
Ad serving & Ad Management Script. Adwords & Adsense Clone.
Inout
Email Marketer
Bulk Mailing & List Management Script. Reach Your Market directly.
Email Marketer
Bulk Mailing & List Management Script. Reach Your Market directly.
Inout
PPC Engine
Powerful Ad management combined with standard Pay Per Click Script.
PPC Engine
Powerful Ad management combined with standard Pay Per Click Script.
Inout
Webmail
Powerful Webmail solution for small business.
Webmail
Powerful Webmail solution for small business.
Inout
Support Desk Manager
Professional customer support & ticketing solution.
Support Desk Manager
Professional customer support & ticketing solution.
Inout
RealEstate
Premium Real Estate Property Management Script. Trulia/Realtor/Zillow Clone.
RealEstate
Premium Real Estate Property Management Script. Trulia/Realtor/Zillow Clone.
Inout
StickBoard
Premium Pin and Board Style Social Photo/Video Sharing Script.
StickBoard
Premium Pin and Board Style Social Photo/Video Sharing Script.
Inout
EasyRooms
Space Rental and Vacation Rental Script. Airbnb Clone Script.
EasyRooms
Space Rental and Vacation Rental Script. Airbnb Clone Script.
Inout
Shopping Cart
Multi-Vendor Shopping cart. Ready for eCommerce.
Shopping Cart
Multi-Vendor Shopping cart. Ready for eCommerce.
Inout
Music
Most powerful Music selling & sharing script on the market.
Music
Most powerful Music selling & sharing script on the market.
Inout
Video
Video Sharing Portal. A YouTube clone with Ads Enabled.
Video
Video Sharing Portal. A YouTube clone with Ads Enabled.
Inout
SmartDeal
Group Deals Script. A Groupon & LivingSocial Clone.
SmartDeal
Group Deals Script. A Groupon & LivingSocial Clone.
Inout
Queryspace
Question & Answer Script.
Queryspace
Question & Answer Script.
Inout
CareerLamp™
Meticulously Designed Job Portal Website. A Monster.com Clone.
CareerLamp™
Meticulously Designed Job Portal Website. A Monster.com Clone.
Inout
Web Portal
Start your own Web Portal.Combine multiple scripts
Web Portal
Start your own Web Portal.Combine multiple scripts
Inout
SocialTiles
Social Media Clone Script. Facebook Clone Script.
SocialTiles
Social Media Clone Script. Facebook Clone Script.
Inout
Article Base
Content Management System (CMS). Blogs, articles and more.
Article Base
Content Management System (CMS). Blogs, articles and more.
Inout
Celebrities
Gossip, News & More. Premium Entertainment Portal
Celebrities
Gossip, News & More. Premium Entertainment Portal
ioMob
Tunes
Most Powerful Music Selling & Sharing Script on the Market.
Tunes
Most Powerful Music Selling & Sharing Script on the Market.
ioMob
Cart
eCommerce Mobile App for small to medium businesses around the world.
Cart
eCommerce Mobile App for small to medium businesses around the world.
ioMob
Rooms
App for easy and flexible Vacation & Space Rentals.
Rooms
App for easy and flexible Vacation & Space Rentals.
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